NZ711776B2 - Mice expressing a limited immunoglobulin light chain repertoire - Google Patents
Mice expressing a limited immunoglobulin light chain repertoire Download PDFInfo
- Publication number
- NZ711776B2 NZ711776B2 NZ711776A NZ71177614A NZ711776B2 NZ 711776 B2 NZ711776 B2 NZ 711776B2 NZ 711776 A NZ711776 A NZ 711776A NZ 71177614 A NZ71177614 A NZ 71177614A NZ 711776 B2 NZ711776 B2 NZ 711776B2
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- human
- mouse
- light chain
- gene segment
- immunoglobulin
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Abstract
genetically modified mouse is provided, wherein the mouse expresses an immunoglobulin light chain repertoire characterized by a limited number of light chain variable domains. Mice are provided that present a choice of two human light chain variable gene segments such that the immunoglobulin light chains expresses by the mouse comprise one of the two human light chain variable gene segments. In a particular embodiment, a mouse comprises in its germline genome exactly two unrearranged human V? gene segments and five unrearranged human J? gene segments operably linked to a mouse light chain constant region at the endogenous kappa light chain loci of the mouse, wherein the exactly two unrearranged human V? gene segments are a human V?1-39 gene segment and a human V?3-20 gene segment. Methods for making bispecific antibodies having universal light chains using mice as described herein, including human light chain variable regions, are provided. Methods for making human variable regions suitable for use in multispecific binding proteins, e.g., bispecific antibodies, and host cells are provided. chains expresses by the mouse comprise one of the two human light chain variable gene segments. In a particular embodiment, a mouse comprises in its germline genome exactly two unrearranged human V? gene segments and five unrearranged human J? gene segments operably linked to a mouse light chain constant region at the endogenous kappa light chain loci of the mouse, wherein the exactly two unrearranged human V? gene segments are a human V?1-39 gene segment and a human V?3-20 gene segment. Methods for making bispecific antibodies having universal light chains using mice as described herein, including human light chain variable regions, are provided. Methods for making human variable regions suitable for use in multispecific binding proteins, e.g., bispecific antibodies, and host cells are provided.
Description
(12) Granted patent specificaon (19) NZ (11) 711776 (13) B2
(47) Publicaon date: 2022.01.28
(54) MICE EXPRESSING A LIMITED IMMUNOGLOBULIN LIGHT CHAIN REPERTOIRE
(51) Internaonal Patent Classificaon(s):
A01K 67/027 C12N 15/85 C07K 16/00 C07K 16/46
MICE EXPRESSING A LIMITED IMMUNOGLOBULIN LIGHT CHAIN REPERTOIRE
CROSS-REFERENCE TO RELATED APPLICATIONS
This application claims benefit under 35 U.S.C § 119(e) of U.S. Patent
Application Serial No. 13/798,455, filed March 13, 2013, which application is hereby
incorporated by reference in its entirety.
SEQUENCE LISTING
The present application makes reference to a sequence listing submitted in
electronic form as an ascii .txt file named “2010794-0550_ST25” on March 13, 2014. The
.txt file was generated on March 11, 2014 and is 33 kb in size.
FIELD
A genetically modified mouse is provided that expresses antibodies having a
common human variable/mouse constant light chain associated with diverse human
variable/mouse constant heavy chains. A method for making a human bispecific antibody
from human variable region gene sequences of B cells of the mouse is provided.
BACKGROUND
Antibodies typically comprise a homodimeric heavy chain component, wherein
each heavy chain monomer is associated with an identical light chain. Antibodies having a
heterodimeric heavy chain component (e.g., bispecific antibodies) are desirable as
therapeutic antibodies. But making bispecific antibodies having a suitable light chain
component that can satisfactorily associate with each of the heavy chains of a bispecific
antibody has proved problematic.
In one approach, a light chain might be selected by surveying usage statistics for
all light chain variable domains, identifying the most frequently employed light chain in
human antibodies, and pairing that light chain in vitro with the two heavy chains of differing
specificity.
In another approach, a light chain might be selected by observing light chain
sequences in a phage display library (e.g., a phage display library comprising human light
chain variable region sequences, e.g., a human scFv library) and selecting the most
commonly used light chain variable region from the library. The light chain can then be
tested on the two different heavy chains of interest.
In another approach, a light chain might be selected by assaying a phage display
library of light chain variable sequences using the heavy chain variable sequences of both
heavy chains of interest as probes. A light chain that associates with both heavy chain
variable sequences might be selected as a light chain for the heavy chains.
In another approach, a candidate light chain might be aligned with the heavy
chains’ cognate light chains, and modifications are made in the light chain to more closely
match sequence characteristics common to the cognate light chains of both heavy chains. If
the chances of immunogenicity need to be minimized, the modifications preferably result in
sequences that are present in known human light chain sequences, such that proteolytic
processing is unlikely to generate a T cell epitope based on parameters and methods known
in the art for assessing the likelihood of immunogenicity (i.e., in silico as well as wet assays).
All of the above approaches rely on in vitro methods that subsume a number of a
priori restraints, e.g., sequence identity, ability to associate with specific pre-selected heavy
chains, etc. There is a need in the art for compositions and methods that do not rely on
manipulating in vitro conditions, but that instead employ more biologically sensible
approaches to making human epitope-binding proteins that include a common light chain.
SUMMARY
Genetically modified mice that express human immunoglobulin heavy and light
chain variable domains, wherein the mice have a limited light chain variable repertoire, are
provided. A biological system for generating a human light chain variable domain that
associates and expresses with a diverse repertoire of affinity-matured human heavy chain
variable domains is provided. Methods for making binding proteins comprising
immunoglobulin variable domains are provided, comprising immunizing mice that have a
limited immunoglobulin light chain repertoire with an antigen of interest, and employing an
immunoglobulin variable region gene sequence of the mouse in a binding protein that
specifically binds the antigen of interest. Methods include methods for making human
immunoglobulin heavy chain variable domains suitable for use in making multi-specific
antigen-binding proteins.
Genetically engineered mice are provided that select suitable affinity-matured
human immunoglobulin heavy chain variable domains derived from a repertoire of
unrearranged human heavy chain variable region gene segments, wherein the affinity-
matured human heavy chain variable domains associate and express with a single human
light chain variable domain derived from one human light chain variable region gene
segment. Genetically engineered mice that present a choice of two human light chain
variable region gene segments are also provided. In various aspects, the one or two gene
segments include human V 1-39 and/or human V 3-20.
Genetically engineered mice are provided that express a limited repertoire of
human light chain variable domains, or a single human light chain variable domain, from a
limited repertoire of human light chain variable region gene segments. In some
embodiments, provided mice are genetically engineered to include a single unrearranged
human light chain variable region gene segment (or two human light chain variable region
gene segments) that rearranges to form a rearranged human light chain variable region
gene (or two rearranged light chain variable region genes) that expresses a single light chain
(or that express either or both of two light chains). The rearranged human light chain
variable domains are capable of pairing with a plurality of affinity-matured human heavy
chains selected by the mice, wherein the heavy chain variable regions specifically bind
different epitopes.
Genetically engineered mice are provided that express a limited repertoire of
human light chain variable domains, or a single human light chain variable domain, from a
limited repertoire of human light chain variable region sequences. In some embodiments,
provided mice are genetically engineered to include a single V/J human light chain sequence
(or two V/J sequences) that express a variable region of a single light chain (or that express
either or both of two variable regions). A light chain comprising the variable sequence is
capable of pairing with a plurality of affinity-matured human heavy chains clonally selected
by the mice, wherein the heavy chain variable regions specifically bind different epitopes.
In a first aspect of the present invention, there is provided a mouse comprising, in
its germline genome: exactly two unrearranged human V gene segments and five
unrearranged human J gene segments operably linked to a mouse light chain constant
region at the endogenous kappa light chain loci of the mouse, wherein the exactly two
unrearranged human Vκ gene segments are a human Vκ1-39 gene segment and a human
Vκ3-20 gene segment; and one or more unrearranged human VH gene segments, one or
more unrearranged human DH gene segments, and one or more unrearranged human JH
gene segments operably linked to a mouse heavy chain constant region at the endogenous
heavy chain loci of the mouse; wherein the unrearranged human heavy chain and kappa
light chain gene segments are capable of rearranging and encoding human variable
domains of an antibody, and further wherein the mouse does not comprise an endogenous
V gene segment that is capable of rearranging to form an immunoglobulin light chain
variable region.
In a second aspect of the present invention, there is provided a method for
making an antibody comprising: expressing in a single cell: (a) a first nucleic acid
sequence that encodes a first immunoglobulin heavy chain, the first nucleic acid sequence
comprising a first human immunoglobulin heavy chain variable region sequence operably
linked to a human immunoglobulin heavy chain constant region sequence, wherein the first
human immunoglobulin heavy chain variable region sequence is identified from a B cell of a
first mouse, and wherein the first mouse has been immunized with a first antigen of interest
including a first epitope, and the first mouse comprises in its germline genome: (i) exactly two
unrearranged human immunoglobulin V gene segments and five unrearranged human
immunoglobulin J gene segments operably linked to a mouse immunoglobulin light chain
constant region sequence at the endogenous kappa light chain loci of the mouse, wherein
the two unrearranged human immunoglobulin V gene segments are a human V 1-39 gene
segment and a human V 3-20 gene segment; and (ii) one or more unrearranged
human immunoglobulin VH gene segments, one or more unrearranged human
immunoglobulin DH gene segments, and one or more unrearranged human immunoglobulin
JH gene segments operably linked to a mouse immunoglobulin heavy chain constant region
sequence at the endogenous heavy chain loci of the mouse; wherein the unrearranged
human heavy chain and kappa light chain immunoglobulin gene segments of the first mouse
are capable of rearranging and encoding human immunoglobulin variable domains of an
antibody, wherein the first mouse does not comprise an endogenous immunoglobulin V
gene segment that is capable of rearranging to form an immunoglobulin light chain variable
region sequence, and wherein the first human immunoglobulin heavy chain variable region
sequence encodes a first human immunoglobulin heavy chain variable domain that
recognizes the first epitope; and (b) a second nucleic acid sequence that encodes an
immunoglobulin light chain, the second nucleic acid sequence comprising a human
immunoglobulin kappa light chain variable region sequence fused with a human
immunoglobulin light chain constant region sequence, wherein the human immunoglobulin
kappa light chain variable region sequence comprises a human V 1-39 gene segment, a
human V 3-20 gene segment, or a somatically hypermutated version thereof; maintaining
the cell under conditions sufficient to express a fully human antibody; and isolating the
antibody.
In one aspect, there may be a genetically modified mouse is provided that
comprises a single human immunoglobulin light chain variable (V ) region gene segment
that is capable of rearranging with a human J gene segment (selected from one or a plurality
of J segments) and encoding a human V domain of an immunoglobulin light chain. In
another aspect, a genetically modified mouse is provided that comprises no more than two
human V gene segments, each of which is capable of rearranging with a human J gene
segment (selected from one or a plurality of J segments) and encoding a human V domain
of an immunoglobulin light chain. In some embodiments, the two human V gene segments
are juxtaposed in the genome of the mouse. In some embodiments, the two human V gene
segments are at different loci (e.g., a heterozygote, comprising a first human V segment at
a first light chain allele, and a second human V segment at a second light chain allele,
wherein the first and the second human V segments are not identical) in the genome of the
mouse. In some embodiments, the two human V gene segments are a human V 1-39
gene segment and a human V 3-20 gene segment. In one embodiment, the human J gene
segment is selected from the group consisting of J 1, J 2, J 3, J 4, J 5, and pairwise
combinations thereof. In various embodiments, a provided genetically engineered mouse is
incapable of expressing an immunoglobulin light chain that contains an endogenous V gene
segment. For example, in some embodiments, a provided genetically engineered mouse
contains a genetic modification that inactivates and/or removes part or all of an endogenous
V gene segment.
In one embodiment, the single human V gene segment is operably linked to a
human J gene segment selected from J 1, J 2, J 3, J 4, and J 5, wherein the single
human V gene segment is capable of rearranging to form a sequence encoding a light
chain variable region gene with any of the one or more human J gene segments.
In one embodiment, a provided genetically modified mouse comprises an
immunoglobulin light chain locus that does not comprise an endogenous mouse V gene
segment that is capable of rearranging to form an immunoglobulin light chain gene, wherein
the V locus contains a single human V gene segment that is capable of rearranging to
encode a V region of a light chain gene. In specific embodiments, the human V gene
segment is a human V 1-39J 5 gene segment or a human V 3-20J 1 gene segment. In
some embodiments, a provided genetically modified mouse comprises a V locus that does
not comprise an endogenous mouse V gene segment that is capable of rearranging to form
an immunoglobulin light chain gene, wherein the V locus comprises no more than two
human V gene segments that are capable of rearranging to encode a V region of a light
chain gene. In some certain embodiments, the no more than two human VL gene segments
are selected from the group consisting of a human V 1-39 gene segment, a human V 3-20
gene segment, and a combination thereof. In some certain embodiments, the no more than
two human V gene segments are a human V 1-39J 5 gene segment and a human V 3-
20J 1 gene segment.
In one aspect, there may be a genetically modified mouse is provided that
comprises a single rearranged (V/J) human immunoglobulin light chain variable (V ) region
(i.e., a V /J region) that encodes a human V domain of an immunoglobulin light chain. In
L L L
another aspect, the mouse comprises no more than two rearranged human V regions that
are capable of encoding a human V domain of an immunoglobulin light chain.
In one embodiment, the V region is a rearranged human V 1-39/J sequence or a
rearranged human V 3-20/J sequence. In one embodiment, the human J segment of the
rearranged V /J sequence is selected from J 1, J 2, J 3, J 4, and J 5. In a specific
embodiment, the V region is a human V 1-39J 5 sequence or a human V 3-20J 1
sequence. In a specific embodiment, the mouse has both a human V 1-39J 5 sequence
and a human V 3-20J 1 sequence.
In one embodiment, the human VL gene segment is operably linked to a human
or mouse leader sequence. In one embodiment, the leader sequence is a mouse leader
sequence. In a specific embodiment, the mouse leader sequence is a mouse V 3-7 leader
sequence. In a specific embodiment, the leader sequence is operably linked to an
unrearranged human V gene segment. In a specific embodiment, the leader sequence is
operably linked to a rearranged human V /J sequence.
In one embodiment, the V gene segment is operably linked to an
immunoglobulin promoter sequence. In one embodiment, the promoter sequence is a
human promoter sequence. In a specific embodiment, the human immunoglobulin promoter
is a human V 3-15 promoter. In a specific embodiment, the promoter is operably linked to
an unrearranged human V gene segment. In a specific embodiment, the promoter is
operably linked to a rearranged human V /J sequence.
In one embodiment, the light chain locus comprises a leader sequence flanked 5’
(with respect to transcriptional direction of a V gene segment) with a human
immunoglobulin promoter and flanked 3’ with a human V gene segment that rearranges
with a human J segment and encodes a V domain of a reverse chimeric light chain
comprising an endogenous mouse light chain constant region (C ). In a specific
embodiment, the V gene segment is at the mouse V locus, and the mouse C is a mouse
C .
In one embodiment, the light chain locus comprises a leader sequence flanked 5’
(with respect to transcriptional direction of a V gene segment) with a human
immunoglobulin promoter and flanked 3’ with a rearranged human V region (V /J
L L L
sequence) and encodes a V domain of a reverse chimeric light chain comprising an
endogenous mouse light chain constant region (C ). In a specific embodiment, the
rearranged human V /J sequence is at the mouse kappa ( ) locus, and the mouse C is a
L L L
mouse C .
In one embodiment, the V locus of the modified mouse is a light chain locus,
and the light chain locus comprises a mouse intronic enhancer, a mouse 3’ enhancer,
or both an intronic enhancer and a 3’ enhancer.
In one embodiment, the mouse comprises a nonfunctional immunoglobulin
lambda ( ) light chain locus. In a specific embodiment, the light chain locus comprises a
deletion of one or more sequences of the locus, wherein the one or more deletions renders
the light chain locus incapable of rearranging to form a light chain gene. In another
embodiment, all or substantially all of the V gene segments of the light chain locus are
deleted.
In one embodiment, mouse makes a light chain that comprises a somatically
mutated V domain derived from a human V gene segment. In one embodiment, the light
chain comprises a somatically mutated V domain derived from a human V gene segment,
and a mouse C region. In one embodiment, the mouse does not express a light chain.
In one embodiment, the genetically modified mouse is capable of somatically
hypermutating the human V region sequence. In a specific embodiment, the mouse
comprises a cell that comprises a rearranged immunoglobulin light chain gene derived from
a human V gene segment that is capable of rearranging and encoding a V domain, and the
rearranged immunoglobulin light chain gene comprises a somatically mutated V domain.
In one embodiment, the mouse comprises a cell that expresses a light chain
comprising a somatically mutated human V domain linked to a mouse C , wherein the light
chain associates with a heavy chain comprising a somatically mutated V domain derived
from a human V gene segment and wherein the heavy chain comprises a mouse heavy
chain constant region (C ). In a specific embodiment, the heavy chain comprises a mouse
C 1, a mouse hinge, a mouse C 2, and a mouse C 3. In a specific embodiment, the heavy
H H H
chain comprises a human C 1, a hinge, a mouse C 2, and a mouse C 3.
H H H
In one embodiment, the mouse comprises a replacement of endogenous mouse
V gene segments with one or more human V gene segments, wherein the human V gene
H H H
segments are operably linked to a mouse C region gene, such that the mouse rearranges
the human V gene segments and expresses a reverse chimeric immunoglobulin heavy
chain that comprises a human V domain and a mouse C . In one embodiment, 90-100% of
unrearranged mouse V gene segments are replaced with at least one unrearranged human
V gene segment. In a specific embodiment, all or substantially all of the endogenous
mouse V gene segments are replaced with at least one unrearranged human V gene
segment. In one embodiment, the replacement is with at least 19, at least 39, or at least 80
or 81 unrearranged human V gene segments. In one embodiment, the replacement is with
at least 12 functional unrearranged human V gene segments, at least 25 functional
unrearranged human V gene segments, or at least 43 functional unrearranged human V
gene segments. In one embodiment, the mouse comprises a replacement of all mouse D
and J segments with at least one unrearranged human D segment and at least one
unrearranged human J segment. In one embodiment, the at least one unrearranged
human D segment is selected from 1-1, D1-7, 1-26, 2-8, 2-15, 3-3, 3-10, 3-16, 3-22, 5-5, 5-
12, 6-6, 6-13, 7-27, and a combination thereof. In one embodiment, the at least one
unrearranged human J segment is selected from 1, 2, 3, 4, 5, 6, and a combination thereof.
In a specific embodiment, the one or more human V gene segment is selected from a 1-2,
1-8, 1-24, 1-69, 2-5, 3-7, 3-9, 3-11, 3-13, 3-15, 3-20, 3-23, 3-30, 3-33, 3-48, 3-53, 4-31, 4-39,
4-59, 5-51, a 6-1 human V gene segment, and a combination thereof.
In one embodiment, the mouse comprises a B cell that expresses a binding
protein that specifically binds an antigen of interest, wherein the binding protein comprises a
light chain derived from a human V 1-39/J 5 rearrangement or a human V 3-20/J 1
rearrangement, and wherein the cell comprises a rearranged immunoglobulin heavy chain
gene derived from a rearrangement of human V gene segments selected from a 1-69, 2-5,
3-13, 3-23, 3-30, 3-33, 3-53, 4-39, 4-59, and 5-51 gene segment. In one embodiment, the
one or more human V gene segments are rearranged with a human heavy chain J gene
segment selected from 1, 2, 3, 4, 5, and 6. In one embodiment, the one or more human V
and J gene segments are rearranged with a human D gene segment selected from 1-1, 1-
7, 1-26, 2-8, 2-15, 3-3, 3-10, 3-16, 3-22, 5-5, 5-12, 6-6, 6-13, and 7-27. In a specific
embodiment, the light chain gene has 1, 2, 3, 4, or 5 or more somatic hypermutations.
In one embodiment, the mouse comprises a B cell that comprises a rearranged
immunoglobulin heavy chain variable region gene sequence comprising a V /D /J region
H H H
selected from 2-5/6-6/1, 2-5/3-22/1, 3-13/6-6/5, 3-23/2-8/4, 3-23/3-3/4, 3-23/3-10/4, 3-23/6-
6/4, 3-23/7-27/4, 3-30/1-1/4, 3-30/1-7/4, 3-30/3-3/3, 3-30/3-3/4, 3-30/3-22/5, 3-30/5-5/2, 3-
/5-12/4, 3-30/6-6/1, 3-30/6-6/3, 3-30/6-6/4, 3-30/6-6/5, 3-30/6-13/4, 3-30/7-27/4, 3-30/7-
27/5, 3-30/7-27/6, 3-33/1-7/4, 3-33/2-15/4, 4-39/1-26/3, 4-59/3-16/3, 4-59/3-16/4, 4-59/3-
22/3, 5-51/3-16/6, 5-51/5-5/3, 5-51/6-13/5, 3-53/1-1/4, 1-69/6-6/5, and 1-69/6-13/4. In a
specific embodiment, the B cell expresses a binding protein comprising a human
immunoglobulin heavy chain variable region fused with a mouse heavy chain constant
region, and a human immunoglobulin light chain variable region fused with a mouse light
chain constant region.
In one embodiment, the rearranged human V region is a human V 1-39J 5
sequence, and the mouse expresses a reverse chimeric light chain comprising (i) a V
domain derived from the human V /J sequence and (ii) a mouse C ; wherein the light chain
L L L
is associated with a reverse chimeric heavy chain comprising (i) a mouse C and (ii) a
somatically mutated human V domain derived from a human V gene segment selected
from a 1-2, 1-8, 1-24, 1-69, 2-5, 3-7, 3-9, 3-11, 3-13, 3-15, 3-20, 3-23, 3-30, 3-33, 3-48, 3-53,
4-31, 4-39, 4-59, 5-51, a 6-1 human V gene segment, and a combination thereof. In one
embodiment, the mouse expresses a light chain that is somatically mutated. In one
embodiment the C is a mouse C . In a specific embodiment, the human V gene segment
is selected from a 2-5, 3-13, 3-23, 3-30, 4-59, 5-51, and 1-69 gene segment. In a specific
embodiment, the somatically mutated human V domain comprises a sequence derived from
a D segment selected from 1-1, 1-7, 2-8, 3-3, 3-10, 3-16, 3-22, 5-5, 5-12, 6-6, 6-13, and 7-
27. In a specific embodiment, the somatically mutated human V domain comprises a
sequence derived from a J segment selected from 1, 2, 3, 4, 5, and 6. In a specific
embodiment, the somatically mutated human V domain is encoded by a rearranged human
V /D /J sequence selected from 2-5/6-6/1, 2-5/3-22/1, 3-13/6-6/5, 3-23/2-8/4, 3-23/3-3/4, 3-
H H H
23/3-10/4, 3-23/6-6/4, 3-23/7-27/4, 3-30/1-1/4, 3-30/1-7/4, 3-30/3-3/4, 3-30/3-22/5, 3-30/5-
/2, 3-30/5-12/4, 3-30/6-6/1, 3-30/6-6/3, 3-30/6-6/4, 3-30/6-6/5, 3-30/6-13/4, 3-30/7-27/4, 3-
/7-27/5, 3-30/7-27/6, 4-59/3-16/3, 4-59/3-16/4, 4-59/3-22/3, 5-51/5-5/3, 1-69/6-6/5, and 1-
69/6-13/4.
In one embodiment, the rearranged human V region is a human V 3-20J 1
sequence, and the mouse expresses a reverse chimeric light chain comprising (i) a V
domain derived from the rearranged human V /J sequence, and (ii) a mouse C ; wherein
L L L
the light chain is associated with a reverse chimeric heavy chain comprising (i) a mouse C ,
and (ii) a somatically mutated human V derived from a human V gene segment selected
from a 1-2, 1-8, 1-24, 1-69, 2-5, 3-7, 3-9, 3-11, 3-13, 3-15, 3-20, 3-23, 3-30, 3-33, 3-48, 3-53,
4-31, 4-39, 4-59, 5-51, a 6-1 human V gene segment, and a combination thereof. In one
embodiment, the mouse expresses a light chain that is somatically mutated. In one
embodiment the C is a mouse C . In a specific embodiment, the human V gene segment
is selected from a 3-30, 3-33, 3-53, 4-39, and 5-51 gene segment. In a specific
embodiment, the somatically mutated human V domain comprises a sequence derived from
a D segment selected from 1-1, 1-7, 1-26, 2-15, 3-3, 3-16, and 6-13. In a specific
embodiment, the somatically mutated human V domain comprises a sequence derived from
a J segment selected from 3, 4, 5, and 6. In a specific embodiment, the somatically
mutated human V domain is encoded by a rearranged human V /D /J sequence selected
H H H H
from 3-30/1-1/4, 3-30/3-3/3, 3-33/1-7/4, 3-33/2-15/4, 4-39/1-26/3, 5-51/3-16/6, 5-51/6-13/5,
and 3-53/1-1/4.
In one embodiment, the mouse comprises both a rearranged human V 1-39J 5
sequence and a rearranged human V 3-20J 1 sequence, and the mouse expresses a
reverse chimeric light chain comprising (i) a V domain derived from the human V 1-39J 5
sequence or the human V 3-20J 1 sequence, and (ii) a mouse C ; wherein the light chain is
associated with a reverse chimeric heavy chain comprising (i) a mouse C , and (ii) a
somatically mutated human V derived from a human V gene segment selected from a 1-2,
1-8, 1-24, 1-69, 2-5, 3-7, 3-9, 3-11, 3-13, 3-15, 3-20, 3-23, 3-30, 3-33, 3-48, 3-53, 4-31, 4-39,
4-59, 5-51, a 6-1 human V gene segment, and a combination thereof. In one embodiment,
the mouse expresses a light chain that is somatically mutated. In one embodiment the C is
a mouse C .
In one embodiment, 90-100% of the endogenous unrearranged mouse V gene
segments are replaced with at least one unrearranged human V gene segment. In a
specific embodiment, all or substantially all of the endogenous unrearranged mouse V gene
segments are replaced with at least one unrearranged human V gene segment. In one
embodiment, the replacement is with at least 18, at least 39, at least 80, or 81 unrearranged
human V gene segments. In one embodiment, the replacement is with at least 12
functional unrearranged human V gene segments, at least 25 functional unrearranged
human V gene segments, or at least 43 unrearranged human V gene segments.
In one embodiment, the genetically modified mouse is a C57BL strain, in a
specific embodiment selected from C57BL/A, C57BL/An, C57BL/GrFa, C57BL/KaLwN,
C57BL/6, C57BL/6J, C57BL/6ByJ, C57BL/6NJ, C57BL/10, C57BL/10ScSn, C57BL/10Cr,
and C57BL/Ola. In a specific embodiment, the genetically modified mouse is a mix of an
aforementioned 129 strain and an aforementioned C57BL/6 strain. In another specific
embodiment, the mouse is a mix of aforementioned 129 strains, or a mix of aforementioned
BL/6 strains. In a specific embodiment, the 129 strain of the mix is a 129S6 (129/SvEvTac)
strain.
In one embodiment, the mouse expresses a reverse chimeric antibody
comprising a light chain that comprises a mouse C and a somatically mutated human V
domain derived from a rearranged human V 1-39J 5 sequence or a rearranged human
V 3-20J 1 sequence, and a heavy chain that comprises a mouse C and a somatically
mutated human V domain derived from a human V gene segment selected from a 1-2, 1-
8, 1-24, 1-69, 2-5, 3-7, 3-9, 3-11, 3-13, 3-15, 3-20, 3-23, 3-30, 3-33, 3-48, 3-53, 4-31, 4-39,
4-59, 5-51, and a 6-1 human V gene segment, wherein the mouse does not express a fully
mouse antibody and does not express a fully human antibody. In one embodiment the
mouse comprises a light chain locus that comprises a replacement of endogenous mouse
light chain gene segments with the rearranged human V 1-39J 5 sequence or the
rearranged human V 3-20J 1 sequence, and comprises a replacement of all or substantially
all endogenous mouse V gene segments with a complete or substantially complete
repertoire of human V gene segments.
In one aspect, there may be a population of antigen-specific antibodies derived
from a mouse as described herein is provided, wherein the antibodies comprise a light chain
gene derived from a human V 1-39/J 5 rearrangement or a human V 3-20/J 1
rearrangement, and wherein the antibodies comprise a rearranged immunoglobulin heavy
chain gene derived from a rearrangement of a human V gene segment selected from a 1-2,
1-3, 1-8, 1-18, 1-24, 1-46, 1-58, 1-69, 2-5, 2-26, 2-70, 3-7, 3-9, 3-11, 3-13, 3-15, 3-16, 3-20,
3-21, 3-23, 3-30, 3-33, 3-43, 3-48, 3-53, 3-64, 3-72, 3-73, 4-31, 4-34, 4-39, 4-59, 5-51, and a
6-1 human V gene segment. In one embodiment, the one or more human V gene
segments are rearranged with a human heavy chain J gene segment selected from 1, 2, 3,
4, 5, and 6. In a specific embodiment, the light chain has 1, 2, 3, 4, or 5 or more somatic
hypermutations.
In one embodiment, the light chain has 1, 2, 3, or 4 somatic hypermutations. In
one embodiment, the light chain gene has 1 or 2 mutations. In various embodiments, the
light chain gene is capable of incurring multiple mutations along its sequence.
In one embodiment, the light chain is derived from a human V 1-39/J 5
rearrangement and the light chain has at least one or no more than four somatic
hypermutations. In one embodiment, the light chain comprises at least two somatic
hypermutations. In one embodiment, the light chain comprises at least three somatic
hypermutations. In one embodiment, the light chain comprises at least four somatic
hypermutations. In a specific embodiment, at least one such somatic hypermutation is
present in one or more framework regions (FWs) of the light chain. In a specific
embodiment, at least one such somatic hypermutation is present in one or more
complementarity determining regions (CDRs) of the light chain. In a specific embodiment, at
least one such somatic hypermutation is present in one or more FWs and/or one or more
CDRs of the light chain. In various embodiments, the framework regions are selected from
framework 1 (FW1), framework 2 (FW2), framework 3 (FW3), and/or a combination thereof.
In various embodiments, the CDRs are selected from CDR1, CDR2, CDR3, and/or a
combination thereof.
In one embodiment, the heavy chain comprises at least one mutation in one or
more FWs or one or more CDRs. In one embodiment, the heavy chain comprises at least
one mutation in one or more FWs and one or more CDRs. In one embodiment, the heavy
chain comprises at least two mutations in one or more FWs and one or more CDRs. In one
embodiment, the heavy chain comprises at least three mutations in one or more FWs and
one or more CDRs. In one embodiment, the heavy chain comprises at least four mutations
in one or more FWs and one or more CDRs. In one embodiment, the heavy chain
comprises at least five or more than five mutations in one or more FWs and one or more
CDRs; in a specific embodiment, the heavy chain comprises at least five or more than five
mutations in two FWs; in a specific embodiment, the heavy chain comprises at least five or
more than five mutations in one FW and one CDR.
In one embodiment, the light chain is derived from a human V 1-39/J 5
rearrangement and about 9% of the V 1-39/J 5-derived light chains have at least one
mutation present in FW1; in one embodiment, at least 9% of the light chains comprise one
mutation present in FW1. In one embodiment, the light chain is derived from a human V 1-
39/J 5 rearrangement and about 25% of the V 1-39/J 5-derived light chains have at least
one or no more than two mutations present in CDR1; in one embodiment, at least 19% of the
light chains have one mutation present in CDR1; in one embodiment, at least 5% of the light
chains have two mutations present in CDR1.
In one embodiment, the light chain is derived from a human V 1-39/J 5
rearrangement and about 20% of the V 1-39/J 5-derived light chains have at least one or
no more than three mutations present in FW2; in one embodiment, at least 17% of the light
chains have one mutation present in FW2; in one embodiment, at least 1% of the light
chains have two mutations present in FW2; in one embodiment, at least 1% of the light
chains have three mutations present in FW2.
In one embodiment, the light chain is derived from a human V 1-39/J 5
rearrangement and about 10% of the V 1-39/J 5-derived light chains have at least one or
no more than two mutations present in CDR2; in one embodiment, at least 10% of the light
chains have one mutation present in CDR2; in one embodiment, at least 1% of the light
chains have two mutations present in CDR2.
In one embodiment, the light chain is derived from a human V 1-39/J 5
rearrangement and about 29% of the V 1-39/J 5-derived light chains have at least one or
no more than four mutations present in FW3; in one embodiment, at least 21% of the light
chains have one mutation present in FW3; in one embodiment, at least 5% of the light
chains have two mutations present in FW3; in one embodiment, at least 2% of the light
chains have three mutations present in FW3; in one embodiment, at least 2% of the light
chains have four mutations present in FW3.
In one embodiment, the light chain is derived from a human V 1-39/J 5
rearrangement and about 37% of the V 1-39/J 5-derived light chains have at least one or
no more than four mutations present in CDR3; in one embodiment, at least 27% of the light
chains have one mutation present in CDR3; in one embodiment, at least 8% of the light
chains have two mutations present in CDR3; in one embodiment, at least 1% of the light
chains have three mutations present in CDR3; in one embodiment, at least 1% of the light
chains have four mutations present in CDR3.
In one embodiment, a population of antigen-specific antibodies derived from a
mouse as described herein is provided, wherein the antibodies comprise a light chain
derived from a human V 1-39/J 5 rearrangement and about 9% of the V 1-39/J 5-derived
light chains have one or more mutations present in FW1, about 25% of the V 1-39/J 5-
derived light chains have one or more mutations present in CDR1, about 20% of the V 1-
39/J 5-derived light chains have one or more mutations present in FW2, about 10% of the
V 1-39/J 5-derived light chains have one or more mutations present in CDR2, about 29% of
the V 1-39/J 5-derived light chains have one or more mutations present in FW3, and about
37% of the V 1-39/J 5-derived light chains have one or more mutations present in CDR3.
In one embodiment, the light chain is derived from a human V 1-39/J 5
rearrangement and about 35% of the heavy chains have at least one mutation present in
FW1; in one embodiment, at least 25% of the heavy chains have one mutation present in
FW1; in one embodiment, at least 9 % of the heavy chains have two mutations present in
FW1; in one embodiment, at least 1% of the heavy chains have three mutations present in
FW1; in one embodiment, at least 1% of the heavy chains have more than five mutations
present in FW1.
In one embodiment, the light chain is derived from a human V 1-39/J 5
rearrangement and about 92% of the heavy chains have at least one or no more than four
mutations present in CDR1; in one embodiment, at least 92% of the heavy chains have at
least one, at least two, at least three, or at least four mutations present in CDR1; in one
embodiment, at least 26% of the heavy chains have one mutation present in CDR1; in one
embodiment, at least 44% of the heavy chains have two mutations present in CDR1; in one
embodiment, at least 19% of the heavy chains have three mutations present in CDR1; in one
embodiment, at least 3% of the heavy chains have four mutations present in CDR1.
In one embodiment, the light chain is derived from a human V 1-39/J 5
rearrangement and about 66% of the heavy chains have at least one or no more than three
mutations present in FW2; in one embodiment, at least 66% of the heavy chains have at
least one, at least two, or at least three mutations present in FW2; in one embodiment, at
least 35% of the heavy chains have one mutation present in FW2; in one embodiment, at
least 23% of the heavy chains have two mutations present in FW2; in one embodiment, at
least 8% of the heavy chains have three mutations present in FW2.
In one embodiment, the light chain is derived from a human V 1-39/J 5
rearrangement and about 70% of the heavy chains have at least one or no more than four
mutations present in CDR2; in one embodiment, at least 70% of the heavy chains have at
least two, at least three, or at least four mutations present in CDR2; in one embodiment, at
least 34% have one mutation present in CDR2; in one embodiment, at least 20% of the
heavy chains have two mutations present in CDR2; in one embodiment, at least 12% of the
heavy chains have three mutations present in CDR2; in one embodiment, at least 5% of the
heavy chains have four mutations present in CDR2.
In one embodiment, the light chain is derived from a human V 1-39/J 5
rearrangement and about 91% of the heavy chains have at least one or up to five or more
mutations present in FW3; in one embodiment, at least 91% of the heavy chains have at
least two, at least three, at least four, or at least five or more mutations present in FW3; in
one embodiment, at least 19% of the heavy chains have one mutation present in FW3; in
one embodiment, at least 33% of the heavy chains have two mutations present in FW3; in
one embodiment, at least 22% of the heavy chains have three mutations present in FW3; in
one embodiment, at least 11% of the heavy chains have four mutations present in FW3; in
one embodiment, at least 7% of the heavy chains have five or more mutations present in
FW3.
In one embodiment, the light chain is derived from a human V 1-39/J 5
rearrangement and about 63% of the heavy chains have at least one or no more than two
mutations present in CDR3; in one embodiment, at least 63% of the heavy chains have at
one mutation present in CDR3; in one embodiment, at least 54% of the heavy chains have
one mutation present in CDR3; in one embodiment, at least 9% of the heavy chains have
two mutations present in CDR3.
In one embodiment, a population of antigen-specific antibodies derived from a
mouse as described herein is provided, wherein the antibodies comprise a light chain
derived from a human V 1-39/J 5 rearrangement and at least 35% of the heavy chains have
one or more mutations present in FW1, about 92% of the heavy chains have one or more
mutations present in CDR1, about 66% of the heavy chains have one or more mutations
present in FW2, about 70% of the heavy chains have one or more mutations present in
CDR2, about 91% of the heavy chains have one or more mutations present in FW3, and
about 63% of the heavy chains have one or more mutations present in CDR3.
In one embodiment, the light chain is derived from a human V 3-20/J 1
rearrangement and the light chain gene has at least one or no more than two somatic
hypermutations; in one embodiment, the light chain gene has at least two, at least three, at
least four or more somatic hypermutations. In a specific embodiment, the mutations are
present in one or more framework regions of the light chain. In a specific embodiment, the
mutations are present in one or more CDR regions of the light chain. In a specific
embodiment, the mutations are present in one or more framework regions and/or one or
more CDR regions of the light chain. In various embodiments, the framework regions are
selected from framework 1 (FW1), framework 2 (FW2), framework 3 (FW3), and/or a
combination thereof.
In one embodiment, the light chain is derived from a human V 3-20/J 1
rearrangement and about 10% of the V 3-20/J 1-derived light chains have at least one
mutation present in FW1; in one embodiment, at least 10% of the light chains have one
mutation in FW1.
In one embodiment, the light chain is derived from a human V 3-20/J 1
rearrangement and about 53% of the V 3-20/J 1-derived light chains have at least one or
no more than two mutations present in CDR1; in one embodiment, at least 27% of the light
chains have one or more mutations in CDR1; in one embodiment, about 54% of the light
chains have one or two mutations present in CDR1.
In one embodiment, the light chain is derived from a human V 3-20/J 1
rearrangement and about 6% of the V 3-20/J 1-derived light chains have at least one or no
more than two mutations present in FW2; in one embodiment, at least 6% of light chains
have at least one mutation present in FW2; in one embodiment, at least 3% of the light
chains have one mutation present in FW2; in one embodiment, at least 3% of the light
chains have two mutations present in FW2.
In one embodiment, the light chain is derived from a human V 3-20/J 1
rearrangement and at least about 3% of the V 3-20/J 1-derived light chains have at least
one mutation present in CDR2; in one embodiment, at least 3% of the light chains have one
mutation in CDR2.
In one embodiment, the light chain is derived from a human V 3-20/J 1
rearrangement and about 17% or more of the V 3-20/J 1-derived light chains have at least
one or no more than two mutations present in FW3; in one embodiment, at least 20% of the
light chain have one mutation present in FW3; in one embodiment, at least 17% of the light
chains have two mutations present in FW3.
In one embodiment, the light chain is derived from a human V 3-20/J 1
rearrangement and at least 43% of the V 3-20/J 1-derived light chains have at least one
mutation present in CDR3; in one embodiment, at least 43% of the light chains have one
mutation in CDR3.
In one embodiment, a population of antigen-specific antibodies derived from a
mouse as described herein is provided, wherein the antibodies comprise a light chain
derived from a human V 3-20/J 1 rearrangement and about 10% of the V 3-20/J 1-derived
light chains have one or more mutations present in at least, about 53% of the V 3-20/J 1-
derived light chains have one or more mutations present in CDR1, about 6% of the V 3-
/J 1-derived light chains have one or more mutations present in FW2, about 3% of the
V 3-20/J 1-derived light chains have one or more mutations present in CDR2, about 37% of
the V 3-20/J 1-derived light chains have one or more mutations present in FW3, and about
43% of the V 3-20/J 1-derived light chains have one or more mutations present in CDR3.
In one embodiment, the light chain is derived from a human V 3-20/J 1
rearrangement and about 43% of the heavy chains have at least one or no more than two
mutations present in FW1; in one embodiment, at least 41% of the heavy chains have at
least one mutation present in FW1; in one embodiment, about 41% of the heavy chains have
one mutation present in FW1; in one embodiment, about 2% of the heavy chains have two
mutations present in FW1.
In one embodiment, the light chain is derived from a human V 3-20/J 1
rearrangement and about 92% of the heavy chains have at least one or no more than four
mutations present in CDR1; in one embodiment, at least 43% of heavy chains have at least
one mutation present in CDR1; in one embodiment, at least 25% of heavy chains have at
least two mutations present in CDR1; in one embodiment, at least 15% of heavy chains have
at least 3 mutations present in CDR1; in one embodiment, at least 10% of heavy chains
have 4 or more mutations present in CDR1.
In one embodiment, the light chain is derived from a human V 3-20/J 1
rearrangement and about 46% of the heavy chains have at least one or no more than three
mutations present in FW2; in one embodiment, at least 34% of heavy chains have at least
one mutation present in FW2; in one embodiment, at least 10% of heavy chains have two or
more mutations present in FW2; in one embodiment, at least 2% of heavy chains have three
or more mutations present in FW2.
In one embodiment, the light chain is derived from a human V 3-20/J 1
rearrangement and about 84% of the heavy chains have at least one or up to five or more
than five mutations present in CDR2; in one embodiment, at least 39% of the heavy chains
have one or more mutations present in CDR2; in one embodiment, at least 18% of the heavy
chains have two or more mutations present in CDR2; in one embodiment, at least 21% of
the heavy chains have three or more mutations present in CDR2; in one embodiment, at
least 3% of the heavy chains have four or more mutations present in CDR2; in one
embodiment, at least 2% of the heavy chains have five or more mutations present in CDR2.
In one embodiment, the light chain is derived from a human V 3-20/J 1
rearrangement and about 92% of the heavy chains have at least one or up to five or more
than five mutations present in FW3; in one embodiment, at least 21% of the light chains
have at least one mutation present in FW3; in one embodiment, at least 20% of heavy
chains have at least two mutations present in FW3; in one embodiment, at least 13% of the
heavy chains have at least three mutations present in FW3; in one embodiment, at least
% of the heavy chains have at least four mutations in FW3; in one embodiment, at least
18% of the heavy chains have at lest 5 mutations in FW3.
In one embodiment, the light chain is derived from a human V 3-20/J 1
rearrangement and about 7% of the heavy chains have at least one mutation present in
CDR3; in one embodiment, about 7% of the heavy chains have one mutation in CDR3.
In one embodiment, a population of antigen-specific antibodies derived from a
mouse as described herein is provided, wherein the antibodies comprise a light chain
derived from a human V 3-20/J 1 rearrangement and about 43% of the heavy chains have
one or more mutations present in FW1, about 92% of the heavy chains have one or more
mutations present in CDR1, about 46% of the heavy chains have one or more mutations
present in FW2, about 84% of the heavy chains have one or more mutations present in
CDR2, about 92% of the heavy chains have one or more mutations present in FW3, and
about 7% of the heavy chains have one or more mutations present in CDR3.
In one aspect, there may be a mouse that expresses an immunoglobulin light
chain from a rearranged immunoglobulin light chain sequence is provided, wherein the
rearranged immunoglobulin light chain sequence is present in the germline of the mouse,
wherein the immunoglobulin light chain comprises a human variable sequence. In one
embodiment, the germline of the mouse comprises a rearranged immunoglobulin light chain
sequence that is derived from the same V segment and the same J segment as all non-
surrogate light chain sequences present in every B cell of the mouse that comprises a
rearranged light chain sequence.
In one embodiment, the germline of the mouse lacks a functional unrearranged
immunoglobulin light chain V gene segment. In one embodiment, the germline of the mouse
lacks a functional unrearranged immunoglobulin light chain J gene segment.
In one embodiment, the germline of the mouse comprises no more than one, no
more than two, or no more than three rearranged (V/J) light chain sequences.
In one embodiment, the rearranged V/J sequence comprises a light chain
sequence. In a specific embodiment, the light chain sequence is a human light chain
sequence. In a specific embodiment, the light chain sequence is selected from a human
V 1-39/J sequence, a human V 3-20/J sequence, and a combination thereof. In a specific
embodiment, the light chain sequence is a human V 1-39/J 5 sequence. In a specific
embodiment, the light chain sequence is a human V 3-20/J 1 sequence.
In one embodiment, the mouse further comprises in its germline a sequence
selected from a mouse intronic enhancer 5’ with respect to the rearranged immunoglobulin
light chain sequence, a mouse 3’ enhancer, and a combination thereof.
In one embodiment, the mouse comprises an unrearranged human V gene
segment, an unrearranged human D gene segment, and an unrearranged human J gene
segment, wherein said V , D , and J gene segments are capable of rearranging to form an
H H H
immunoglobulin heavy chain variable gene sequence operably linked to a heavy chain
constant gene sequence. In one embodiment, the mouse comprises a plurality of human
V , D , and J gene segments. In a specific embodiment, the human V , D , and J gene
H H H H H H
segments replace endogenous mouse V , D , and J gene segments at the endogenous
H H H
mouse immunoglobulin heavy chain locus. In a specific embodiment, the mouse comprises
a replacement of all or substantially all functional mouse V , D , and J gene segments with
H H H
all or substantially all functional human V , D , and J gene segments.
H H H
In one embodiment, the mouse expresses an immunoglobulin light chain that
comprises a mouse constant sequence. In one embodiment, the mouse expresses an
immunoglobulin light chain that comprises a human constant sequence.
In one embodiment, the mouse expresses an immunoglobulin heavy chain that
comprises a mouse sequence selected from a C 1 sequence, a hinge sequence, a C 2
sequence, a C 3 sequence, and a combination thereof.
In one embodiment, the mouse expresses an immunoglobulin heavy chain that
comprises a human sequence selected from a C 1 sequence, a hinge sequence, a C 2
sequence, a C 3 sequence, and a combination thereof.
In one embodiment, the rearranged immunoglobulin light chain sequence in the
germline of the mouse is at an endogenous mouse immunoglobulin light chain locus. In a
specific embodiment, the rearranged immunoglobulin light chain sequence in the germline of
the mouse replaces all or substantially all mouse light chain V and J sequences at the
endogenous mouse immunoglobulin light chain locus.
In one aspect, there may be a mouse is provided that comprises a B cell
population characterized by each B cell that comprises a non-surrogate light chain
sequence, which sequence comprises a rearranged light chain gene that is generated from a
single human V gene segment and a single human J gene segment, wherein the only light
chain variable sequence in the germline of the mouse is a rearranged sequence generated
from the single human V segment and the single human J segment, and wherein each B cell
that comprises the rearranged light chain gene further comprises a gene encoding a cognate
human heavy chain variable domain, and wherein the rearranged light chain gene comprises
at least one, at least two, at least three, or at least four somatic hypermutations.
In some embodiments, a mouse is provided whose mature B cell population is
characterized in that each mature B cell comprises a non-surrogate light chain sequence on
its surface, which sequence comprises a rearranged light chain gene that is generated
through rearrangement of one of two human V gene segments and one of no more than five
human J gene segments, wherein the only light chain variable sequence (V J sequence) in
L L L
the germline of the mouse is a rearranged sequence that is generated through
rearrangement of one of the two human V gene segments and one of the no more than five
human J gene segments, and wherein each B cell that comprises the rearranged light chain
gene further comprises a gene encoding a cognate human heavy chain variable domain,
and wherein the rearranged light chain gene comprises at least one, at least two, at least
three, at least four, or five or more somatic hypermutations. In some embodiments, a
rearranged light chain gene comprises one, two, three, four, or five somatic hypermutations.
In some embodiments, mice as described herein have been immunized with an antigen of
interest, and, in some embodiments, a mature B cell population is enriched with B cells that
bind the antigen of interest.
In some embodiments, a mouse is provided whose mature B cell population is
characterized in that each mature B cell comprises a non-surrogate light chain sequence on
its surface, which sequence comprises a rearranged light chain gene that is generated
through rearrangement of one of two human V gene segments and one of two or more
(e.g., 2, 3, 4, or 5) human J gene segments, wherein the V gene segments consist
essentially of two V gene segments that are not identical and the V locus comprises two or
more (e.g., 2, 3, 4, or 5) human J gene segments, and wherein each B cell that comprises
the rearranged light chain gene further comprises a gene encoding a cognate human heavy
chain variable domain, and wherein the rearranged light chain gene comprises at least one,
at least two, at least three, at least four, or five or more somatic hypermutations. In some
embodiments, a rearranged light chain gene comprises one, two, three, four, or five somatic
hypermutations. In some embodiments, mice as described herein have been immunized
with an antigen of interest, and in some embodiments, a mature B cell population is enriched
with B cells that bind the antigen of interest.
In one aspect, there may be a pluripotent, induced pluripotent, or totipotent cell
derived from a mouse as described herein is provided. In a specific embodiment, the cell is
a mouse embryonic stem (ES) cell.
In one aspect, there may be a tissue derived from a mouse as described herein is
provided. In one embodiment, the tissue is derived from spleen, lymph node or bone
marrow of a mouse as described herein.
In one aspect, there may be a nucleus derived from a mouse as described herein
is provided. In one embodiment, the nucleus is from a diploid cell that is not a B cell.
In one aspect, a mouse cell is provided that is isolated from a mouse as
described herein. In one embodiment, the cell is an ES cell. In one embodiment, the cell is
a lymphocyte. In one embodiment, the lymphocyte is a B cell. In one embodiment, the B
cell expresses a chimeric heavy chain comprising a variable domain derived from a human
gene segment; and a light chain derived from a rearranged human V 1-39/J sequence,
rearranged human V 3-20/J sequence, or a combination thereof; wherein the heavy chain
variable domain is fused to a mouse constant region and the light chain variable domain is
fused to a mouse or a human constant region.
In one aspect, there may be a hybridoma is provided, wherein the hybridoma is
made with a B cell of a mouse as described herein. In a specific embodiment, the B cell is
from a mouse as described herein that has been immunized with an immunogen comprising
an epitope of interest, and the B cell expresses a binding protein that binds the epitope of
interest, the binding protein has a somatically mutated human V domain and a mouse C ,
and has a human V domain derived from a rearranged human V 1-39J 5 or a rearranged
human V 3-20J 1 and a mouse C .
In one aspect, there may be a mouse embryo is provided, wherein the embryo
comprises a donor ES cell that is derived from a mouse as described herein.
In one aspect, there may be a targeting vector is provided, comprising, from 5’ to
3’ in transcriptional direction with reference to the sequences of the 5’ and 3’ mouse
homology arms of the vector, a 5’ mouse homology arm, a human or mouse immunoglobulin
promoter, a human or mouse leader sequence, and a human V region selected from a
rearranged human V 1-39J 5 or a rearranged human V 3-20J 1, and a 3’ mouse homology
arm. In one embodiment, the 5’ and 3’ homology arms target the vector to a sequence 5’
with respect to an enhancer sequence that is present 5’ and proximal to the mouse C gene.
In one embodiment, the promoter is a human immunoglobulin variable region gene segment
promoter. In a specific embodiment, the promoter is a human V 3-15 promoter. In one
embodiment, the leader sequence is a mouse leader sequence. In a specific embodiment,
the mouse leader sequence is a mouse V 3-7 leader sequence.
In one aspect, there may be a targeting vector is provided as described above,
but in place of the 5’ mouse homology arm the human or mouse promoter is flanked 5’ with a
site-specific recombinase recognition site (SRRS), and in place of the 3’ mouse homology
arm the human V region is flanked 3’ with an SRRS.
In one aspect, there may be a reverse chimeric antibody made by a mouse as
described herein, wherein the reverse chimeric antibody comprises a light chain comprising
a human V and a mouse C , and a heavy chain comprising a human V and a mouse C .
L L H H
In one aspect, there may be a method for making an antibody is provided,
comprising expressing in a single cell (a) a first V gene sequence of an immunized mouse
as described herein fused with a human C gene sequence; (b) a V gene sequence of an
immunized mouse as described herein fused with a human C gene sequence; and, (c)
maintaining the cell under conditions sufficient to express a fully human antibody, and
isolating the antibody. In one embodiment, the cell comprises a second V gene sequence
of a second immunized mouse as described herein fused with a human C gene sequence,
the first V gene sequence encodes a V domain that recognizes a first epitope, and the
second V gene sequence encodes a V domain that recognizes a second epitope, wherein
the first epitope and the second epitope are not identical.
In one aspect, there may be a method for making an epitope-binding protein is
provided, comprising exposing a mouse as described herein with an immunogen that
comprises an epitope of interest, maintaining the mouse under conditions sufficient for the
mouse to generate an immunoglobulin molecule that specifically binds the epitope of
interest, and isolating the immunoglobulin molecule that specifically binds the epitope of
interest; wherein the epitope-binding protein comprises a heavy chain that comprises a
somatically mutated human V and a mouse C , associated with a light chain comprising a
mouse C and a human V derived from a rearranged human V 1-39J 5 or a rearranged
human V 3-20J1.
In one aspect, there may be a cell that expresses an epitope-binding protein is
provided, wherein the cell comprises: (a) a human nucleotide sequence encoding a human
V domain that is derived from a rearranged human V 1-39J 5 or a rearranged human V 3-
20J 1, wherein the human nucleotide sequence is fused (directly or through a linker) to a
human immunoglobulin light chain constant domain cDNA sequence (e.g., a human
constant domain DNA sequence); and, (b) a first human V nucleotide sequence encoding a
human V domain derived from a first human V nucleotide sequence, wherein the first
human V nucleotide sequence is fused (directly or through a linker) to a human
immunoglobulin heavy chain constant domain cDNA sequence; wherein the epitope-binding
protein recognizes a first epitope. In one embodiment, the epitope-binding protein binds the
-6 -8
first epitope with a dissociation constant of lower than 10 M, lower than 10 M, lower than
-9 -10 -11 -12
M, lower than 10 M, lower than 10 M, or lower than 10 M.
In one embodiment, the cell comprises a second human nucleotide sequence
encoding a second human V domain, wherein the second human sequence is fused
(directly or through a linker) to a human immunoglobulin heavy chain constant domain cDNA
sequence, and wherein the second human V domain does not specifically recognize the
-6 -5 -4
first epitope (e.g., displays a dissociation constant of, e.g., 10 M, 10 M, 10 M, or higher),
and wherein the epitope-binding protein recognizes the first epitope and the second epitope,
and wherein the first and the second immunoglobulin heavy chains each associate with an
identical light chain of (a).
In one embodiment, the second V domain binds the second epitope with a
-6 -7 -8
dissociation constant that is lower than 10 M, lower than 10 M, lower than 10 M, lower
-9 -10 -11 -12
than 10 M, lower than 10 M, lower than 10 M, or lower than 10 M.
In one embodiment, the epitope-binding protein comprises a first immunoglobulin
heavy chain and a second immunoglobulin heavy chain, each associated with an identical
light chain derived from a rearranged human V region selected from a human V 1-39J 5 or
a human V 3-20J 1, wherein the first immunoglobulin heavy chain binds a first epitope with
a dissociation constant in the nanomolar to picomolar range, the second immunoglobulin
heavy chain binds a second epitope with a dissociation constant in the nanomolar to
picomolar range, the first epitope and the second epitope are not identical, the first
immunoglobulin heavy chain does not bind the second epitope or binds the second epitope
with a dissociation constant weaker than the micromolar range (e.g., the millimolar range),
the second immunoglobulin heavy chain does not bind the first epitope or binds the first
epitope with a dissociation constant weaker than the micromolar range (e.g., the millimolar
range), and one or more of the V , the V of the first immunoglobulin heavy chain, and the
V of the second immunoglobulin heavy chain, are somatically mutated.
In one embodiment, the first immunoglobulin heavy chain comprises a protein A-
binding residue, and the second immunoglobulin heavy chain lacks the protein A-binding
residue.
In one embodiment, the cell is selected from CHO, COS, 293, HeLa, and a retinal
cell expressing a viral nucleic acid sequence (e.g., a PERC.6™ cell).
In one aspect, there may be a reverse chimeric antibody is provided, comprising
a human V and a mouse heavy chain constant domain, a human V and a mouse light
chain constant domain, wherein the antibody is made by a process that comprises
immunizing a mouse as described herein with an immunogen comprising an epitope, and
the antibody specifically binds the epitope of the immunogen with which the mouse was
immunized. In one embodiment, the VL domain is somatically mutated. In one embodiment
the V domain is somatically mutated. In one embodiment, both the V domain and the V
H L H
domain are somatically mutated. In one embodiment, the V is linked to a mouse C
domain.
In one aspect, there may be a mouse is provided, comprising human V gene
segments replacing all or substantially all mouse V gene segments at the endogenous
mouse heavy chain locus; no more than one or two rearranged human light chain V /J
sequences selected from a rearranged V 1-39/J and a rearranged V 3-20/J or a
combination thereof, replacing all mouse light chain gene segments; wherein the human
heavy chain variable gene segments are linked to a mouse constant gene, and the
rearranged human light chain sequences are linked to a human or mouse constant gene.
In some embodiments, a mouse is provided, comprising human immunoglobulin
V gene segments replacing all or substantially all mouse immunoglobulin V gene
segments at the endogenous mouse immunoglobulin heavy chain locus; no more than two
unrearranged human immunoglobulin V gene segments and two or more (e.g., 2, 3, 4 or 5)
unrearranged human immunoglobulin J gene segments or five human immunoglobulin J
gene segments, replacing all mouse immunoglobulin light chain gene segments; wherein the
human immunoglobulin VH gene segments are linked to a mouse immunoglobulin constant
gene, and the unrearranged human immunoglobulin V and J gene segments are linked to
a human or non-human immunoglobulin constant gene. In some embodiments, a non-
human constant gene is a mouse immunoglobulin constant gene. In some embodiments, a
non-human immunoglobulin constant gene is a rat immunoglobulin constant gene.
In one aspect, there may be a mouse ES cell comprising a replacement of all or
substantially all mouse heavy chain variable gene segments with human heavy chain
variable gene segments, and no more than one or two rearranged human light chain V /J
sequences, wherein the human heavy chain variable gene segments are linked to a mouse
immunoglobulin heavy chain constant gene, and the rearranged human light chain V /J
sequences are linked to a mouse or human immunoglobulin light chain constant gene. In a
specific embodiment, the light chain constant gene is a mouse constant gene.
In some embodiments, a mouse ES cell is provided, comprising a replacement of
all or substantially all mouse immunoglobulin V gene segments with human immunoglobulin
V gene segments and no more than two unrearranged human immunoglobulin V gene
segments and two or more (e.g., 2, 3, 4, or 5) unrearranged human immunoglobulin J gene
segments, wherein the human immunoglobulin V gene segments are linked to a mouse
immunoglobulin heavy chain constant gene, and the unrearranged human immunoglobulin
V and J gene segments are linked to a non-human or human immunoglobulin light chain
constant gene. In some certain embodiments, the non-human immunoglobulin light chain
constant gene is a mouse immunoglobulin constant gene. In some certain embodiments,
the mouse comprises five unrearranged immunoglobulin J gene segments.
In some embodiments, a mouse is provided, comprising a light chain locus
whose structure is different from that of the reference structure of in that at least
one, and in some embodiments all, mouse V gene segments are replaced by one human V
gene segment or no more than two human V gene segments. In some embodiments,
human V gene segments of a mouse are capable of rearranging to one of two or more
human J gene segments to encode an immunoglobulin V domain of an antibody. In some
embodiments, human V gene segment(s) of a light chain locus of a mouse as described
herein is/are operably linked to two or more (e.g., two, three, four, or five) human J gene
segments.
In some embodiments, a mouse is provided, comprising a light chain locus
whose structure is different from that of the reference structure of in that it does not
contain a nucleotide sequence before rearrangement that encodes an endogenous V gene
segment. In some embodiments, a mouse is provided, comprising a light chain locus whose
structure is different from that of the reference structure of in that it does not contain
a nucleotide sequence before rearrangement that encodes an endogenous J gene
segment. In some embodiments, a mouse is provided, comprising a light chain locus whose
structure is different from that of the reference structure of in that it does not contain
a nucleotide before rearrangement that encodes endogenous V and J gene segments.
In some embodiments, a mouse is provided, comprising a light chain locus
whose structure is different from that of the reference structure of in that it does not
contain a nucleotide sequence after rearrangement that encodes an endogenous V gene
segment. In some embodiments, a mouse is provided, comprising a light chain locus whose
structure is different from that of the reference structure of in that it does not contain
a nucleotide sequence after rearrangement that encodes an endogenous J gene segment.
In some embodiments, a mouse is provided, comprising a light chain locus whose structure
is different from that of the reference structure of in that it does not contain a
nucleotide sequence after rearrangement that encodes endogenous V and J gene
segments.
In some embodiments, a mouse is provided, comprising a light chain locus
whose structure is different from that of the reference structure of in that it contains
no more than two human V gene segments and two or more (e.g., two, three, four, or five)
human J gene segments before rearrangement. In some embodiments, a mouse is
provided, comprising a light chain locus whose structure is different from that of the
reference structure of in that it contains no more than two human VL gene segments
and five human J gene segments before rearrangement.
In some embodiments, a mouse is provided, comprising a light chain locus
whose structure is different from that of the reference structure of in that it contains
no more than two human V gene segments and five or less (e.g., 5, 4, 3, 2, or 1) human J
gene segments after rearrangement. In some embodiments, a mouse is provided,
comprising a light chain locus whose structure is different from that of the reference structure
of in that it contains no more than two human V gene segments and one, two,
three, four, or five human J gene segments after rearrangement.
In some embodiments, a mouse is provided, comprising a light chain locus
whose structure is different from that of the reference structure of in that it contains
one human V gene segment and five or less (e.g., 5, 4, 3, 2, or 1) human J gene segments
after rearrangement. In some embodiments, a mouse is provided, comprising a light chain
locus whose structure is different from that of the reference structure of in that it
contains one human V gene segment and one, two, three, four, or five human J gene
segments after rearrangement.
In various embodiments, human V and J gene segments are human V and J
gene segments. In various embodiments, human V segments are selected from a human
V 1-39 gene segment and a human V 3-20 gene segment. In some embodiments, human
V segments are human V 1-39 and human V 3-20. In some embodiments, human J
segments are selected from a J 1, J 2, J 3, J 4, J 5 gene segment, and a combination
thereof. In some embodiments, human J gene segments are human J 1, J 2, J 3, J 4,
and J 5.
In some embodiments, a mouse is provided, comprising a light chain locus
whose structure is different from that of the reference structure of in that it contains a
structure that is substantially the same as that of the structure of or
before rearrangement. In some embodiments, a mouse is provided, comprising a
light chain locus whose structure is identical to the structure of or before rearrangement.
In one aspect, there may be an antigen-binding protein made by a mouse as
described herein is provided. In a specific embodiment, the antigen-binding protein
comprises a human immunoglobulin heavy chain variable region fused with a mouse
constant region, and a human immunoglobulin light chain variable region derived from a
V 1-39 gene segment or a V 3-20 gene segment, wherein the light chain constant region is
a mouse constant region.
In one aspect, there may be a fully human antigen-binding protein made from an
immunoglobulin variable region gene sequence from a mouse as described herein is
provided, wherein the antigen-binding protein comprises a fully human heavy chain
comprising a human variable region derived from a sequence of a mouse as described
herein, and a fully human light chain comprising a V 1-39 or a V 3-20. In one embodiment,
the light chain variable region comprises one to five somatic mutations. In one embodiment,
the light chain variable region is a cognate light chain variable region that is paired in a B cell
of the mouse with the heavy chain variable region.
In one embodiment, the fully human antigen-binding protein comprises a first
heavy chain and a second heavy chain, wherein the first heavy chain and the second heavy
chain comprise non-identical variable regions independently derived from a mouse as
described herein, and wherein each of the first and second heavy chains express from a
host cell associated with a human light chain derived from a V 1-39 gene segment or a V 3-
gene segment. In one embodiment, the first heavy chain comprises a first heavy chain
variable region that specifically binds a first epitope of a first antigen, and the second heavy
chain comprises a second heavy chain variable region that specifically binds a second
epitope of a second antigen. In a specific embodiment, the first antigen and the second
antigen are different. In a specific embodiment, the first antigen and the second antigen are
the same, and the first epitope and the second epitope are not identical; in a specific
embodiment, binding of the first epitope by a first molecule of the binding protein does not
block binding of the second epitope by a second molecule of the binding protein.
In one aspect, there may be a fully human binding protein derived from a human
immunoglobulin sequence of a mouse as described herein comprises a first immunoglobulin
heavy chain and a second immunoglobulin heavy chain, wherein the first immunoglobulin
heavy chain comprises a first variable region that is not identical to a variable region of the
second immunoglobulin heavy chain, and wherein the first immunoglobulin heavy chain
comprises a wild type protein A binding determinant, and the second heavy chain lacks a
wild type protein A binding determinant. In one embodiment, the first immunoglobulin heavy
chain binds protein A under isolation conditions, and the second immunoglobulin heavy
chain does not bind protein A or binds protein A at least 10-fold, a hundred-fold, or a
thousand-fold weaker than the first immunoglobulin heavy chain binds protein A under
isolation conditions. In a specific embodiment, the first and the second heavy chains are
IgG1 isotypes, wherein the second heavy chain comprises a modification selected from 95R
(EU 435R), 96F (EU 436F), and a combination thereof, and wherein the first heavy chain
lacks such modification.
In one aspect, there may be a method for making a bispecific antigen-binding
protein is provided, comprising exposing a first mouse as described herein to a first antigen
of interest that comprises a first epitope, exposing a second mouse as described herein to a
second antigen of interest that comprises a second epitope, allowing the first and the second
mouse to each mount immune responses to the antigens of interest, identifying in the first
mouse a first human heavy chain variable region that binds the first epitope of the first
antigen of interest, identifying in the second mouse a second human heavy chain variable
region that binds the second epitope of the second antigen of interest, making a first fully
human heavy chain gene that encodes a first heavy chain that binds the first epitope of the
first antigen of interest, making a second fully human heavy chain gene that encodes a
second heavy chain that binds the second epitope of the second antigen of interest,
expressing the first heavy chain and the second heavy chain in a cell that expresses a single
fully human light chain derived from a human V 1-39 or a human V 3-20 gene segment to
form a bispecific antigen-binding protein, and isolating the bispecific antigen-binding protein.
In one embodiment, the first antigen and the second antigen are not identical.
In one embodiment, the first antigen and the second antigen are identical, and
the first epitope and the second epitope are not identical. In one embodiment, binding of the
first heavy chain variable region to the first epitope does not block binding of the second
heavy chain variable region to the second epitope.
In one embodiment, the human light chain when paired with the first heavy chain
specifically binds the first epitope of the first antigen and when paired the second heavy
chain specifically binds the second epitope of the second antigen.
In one embodiment, the first antigen is selected from a soluble antigen and a cell
surface antigen (e.g., a tumor antigen), and the second antigen comprises a cell surface
receptor. In a specific embodiment, the cell surface receptor is an immunoglobulin receptor.
In a specific embodiment, the immunoglobulin receptor is an Fc receptor. In one
embodiment, the first antigen and the second antigen are the same cell surface receptor,
and binding of the first heavy chain to the first epitope does not block binding of the second
heavy chain to the second epitope.
In one embodiment, the light chain variable domain of the light chain comprises 2
to 5 somatic mutations. In one embodiment, the light chain variable domain is a somatically
mutated cognate light chain expressed in a B cell of the first or the second immunized
mouse with either the first or the second heavy chain variable domain. In one embodiment,
the light chain of the cell comprises a germline sequence.
In one embodiment, the first fully human heavy chain bears an amino acid
modification that reduces its affinity to protein A, and the second fully human heavy chain
does not comprise a modification that reduces its affinity to protein A.
In one aspect, there may be a method of preparing a bispecific antibody that
specifically binds to a first and a second antigen is provided, wherein the method comprises
(a) identifying a first nucleic acid sequence that encodes a first human heavy chain variable
(V ) domain that is specific for the first antigen; (b) identifying a second nucleic acid
sequence that encodes a second human heavy chain variable (V ) domain that is specific
for the second antigen; (c) providing a third nucleic acid sequence that encodes a human
light chain variable (V ) region which, when paired with the V region of (a) specifically binds
the first antigen, and when paired with the V region of (b) specifically binds to the second
antigen; (d) culturing a host cell comprising the first, second, and third nucleic acid
sequences to allow expression of the first and second human V regions and the human V
region to form the bispecific antibody; and (d) recovering said bispecific antibody. In various
aspects, the first and second antigens are different from one another. In various aspects the
first and second nucleic acid sequences are isolated from an immunized mouse that
expresses a human immunoglobulin V region from a rearranged immunoglobulin light chain
sequence, wherein the rearranged immunoglobulin sequence is in the germline of the
mouse.
In one embodiment, the human V region is derived from a rearranged human
light chain sequence comprising a human V 1-39 gene segment or a human V 3-20 gene
segment. In a specific embodiment, the rearranged human light chain sequence is a
germline sequence (i.e., does not comprise a somatic hypermutation within the V gene
segment sequence).
In one embodiment, the third nucleic acid sequence is isolated from a mouse that
expresses a human immunoglobulin V region from a rearranged immunoglobulin light chain
sequence in the germline of the mouse. In one embodiment, the rearranged immunoglobulin
light chain sequence comprises a human V 1-39 or human V 3-20 gene segment. In a
specific embodiment, the rearranged immunoglobulin light chain sequence comprises a
human V 1-39 gene segment. In one embodiment, the human immunoglobulin V region is
expressed from a modified endogenous immunoglobulin light chain locus.
In one embodiment, the first and second antigens are present on one molecule.
In one embodiment, the first and second antigens are present on different molecules. In
various embodiments, the first or second nucleic acid sequence comprises a modification
that reduces the affinity of the encoded heavy chain to protein A.
In one embodiment, the first or second nucleic acid sequences comprise a
rearranged human heavy chain variable region sequence comprising a human heavy chain
gene segment selected from V 1-2, V 1-3, V 1-8, V 1-18, V 1-24, V 1-46, V 1-58, V 1-69,
H H H H H H H H
V 2-5, V 2-26, V 2-70, V 3-7, V 3-9, V 3-11, V 3-13, V 3-15, V 3-20, V 3-21, V 3-23, V 3-
H H H H H H H H H H H H
, V 3-33, V 3-43, V 3-48, V 3-53, V 3-64, V 3-72, V 3-73, V 4-31, V 4-34, V 4-39, V 4-
H H H H H H H H H H H
59, V 5-51, and V 6-1. In a specific embodiment, the heavy chain gene segment is V 2-5,
H H H
V 3-23 or V 3-30.
In one aspect, there may be a method of preparing a bispecific antibody that
specifically binds to a first and a second antigen is provided, wherein the method comprises
(a) identifying a first nucleic acid sequence that encodes a first human heavy chain variable
(V ) domain that is specific for the first antigen; (b) identifying a second nucleic acid
sequence that encodes a second human heavy chain variable (V ) domain that is specific
for the second antigen; (c) providing a third nucleic acid sequence that encodes a human
light chain variable (VL) region derived from a human V 1-39 or human V 3-20 gene
segment which, when paired with the V region of (a) specifically binds the first antigen, and
when paired with the V region of (b) specifically binds to the second antigen; (d) culturing a
host cell comprising the first, second, and third nucleic acid sequences to allow expression
of the first and second human V regions and the human V region to form the bispecific
antibody; and (d) recovering said bispecific antibody. In various aspects, the first and
second antigens are different from one another. In various aspects, the first and second
nucleic acid sequences are isolated from an immunized mouse that expresses a human
immunoglobulin V region from a rearranged immunoglobulin sequence that is derived from
a human V 1-39 or human V 3-20 gene segment, wherein the rearranged human V 1-39 or
V 3-30 gene segment is in the germline of the mouse.
In one embodiment, the third nucleic acid sequence is a germline sequence (i.e.,
does not comprise a somatic hypermutation within the V gene segment sequence). In one
embodiment, the third nucleic acid sequence is isolated from the mouse that expresses a
human immunoglobulin V region derived from a human V 1-39 or human V 3-20 gene
segment from a rearranged immunoglobulin light chain sequence in the germline of the
mouse. In a specific embodiment, the third nucleic acid sequence comprises two to five
somatic hypermutations in a complementary determining region (CDR) and/or a framework
region (FWR). In one embodiment, the human immunoglobulin V region is expressed from
a modified endogenous immunoglobulin light chain locus.
In one embodiment, the first and second antigens are present on one molecule.
In one embodiment, the first and second antigens are present on different molecules. In one
embodiment, the first or second nucleic acid sequence comprises a modification that
reduces the affinity of the encoded heavy chain to protein A.
In one embodiment, the first or second nucleic acid sequences comprise a
rearranged human heavy chain variable region sequence comprising a human heavy chain
gene segment selected from V 1-2, V 1-3, V 1-8, V 1-18, V 1-24, V 1-46, V 1-58, V 1-69,
H H H H H H H H
V 2-5, V 2-26, V 2-70, V 3-7, V 3-9, V 3-11, V 3-13, V 3-15, V 3-20, V 3-21, V 3-23, V 3-
H H H H H H H H H H H H
, V 3-33, V 3-43, V 3-48, V 3-53, V 3-64, V 3-72, V 3-73, V 4-31, V 4-34, V 4-39, V 4-
H H H H H H H H H H H
59, V 5-51, and V 6-1. In a specific embodiment, the heavy chain gene segment is V 2-5,
H H H
V 3-23 or V 3-30.
In one aspect, there may be a method for making a bispecific antibody is
provided, comprising exposing a mouse as described herein to an antigen of interest,
allowing the mouse to mount an immune response to the antigen of interest, identifying a
first human heavy chain variable region that binds a first epitope of the antigen of interest,
identifying a second human heavy chain variable region that binds a second epitope of the
antigen of interest, making a first fully human heavy chain gene that encodes the first heavy
chain that binds the first epitope of the antigen of interest, making a second fully human
heavy chain gene that encodes a second heavy chain that binds the second epitope of the
antigen of interest, expressing the first heavy chain and the second heavy chain in a cell that
expresses a single fully human light chain derived from a human V 1-39 or a human V 3-20
gene segment to form a bispecific antibody, and isolating the bispecific antigen-binding
protein.
In one embodiment, the first epitope and the second epitope are not identical. In
one embodiment, binding of the first heavy chain variable region to the first epitope does not
block binding of the second heavy chain variable region to the second epitope. In one
embodiment, the first and second heavy chains are capable of binding the first and second
epitopes simultaneously.
In one embodiment, the bispecific antibody binds the first and second epitopes
simultaneously. In one embodiment, the bispecific antibody binds the first epitope and
second epitope independently.
In one embodiment, the binding response of the bispecific antibody to the antigen
is about 2-fold higher than the binding response of the first heavy chain variable region to the
antigen. In one embodiment, the binding response of the bispecific antibody to the antigen
is about 2-fold higher than the binding response of the second heavy chain variable region to
the antigen. In one embodiment, the binding response of the bispecific antibody to the
antigen is about the same as, or about equal to, the binding response of the first heavy chain
variable region and or the second heavy chain variable region to the antigen.
In one embodiment, the antigen is selected from a soluble antigen, a cell surface
antigen (e.g., a tumor antigen) and a cell surface receptor. In a specific embodiment, the
cell surface receptor is an immunoglobulin receptor. In a specific embodiment, the
immunoglobulin receptor is an Fc receptor.
In one embodiment, the light chain variable domain of the light chain comprises 2
to 5 somatic mutations. In one embodiment, the light chain variable domain is a somatically
mutated cognate light chain expressed in a B cell of the immunized mouse with either the
first or the second heavy chain variable domain.
In one embodiment, the first fully human heavy chain bears an amino acid
modification that reduces its affinity to protein A, and the second fully human heavy chain
does not comprise a modification that reduces its affinity to protein A.
In various embodiments, methods for making bispecific antibodies are enhanced
by employing a common light chain to pair with each heavy chain variable regions of the
bispecific antibodies. In various embodiments, employing a common light chain as
described herein reduces the number of inappropriate species of immunoglobulins lacking
bispecificity as compared to employing original cognate light chains. In various
embodiments, the heavy chain variable regions of the bispecific antibodies are identified
from monospecific antibodies comprising a common light chain. In various embodiments,
the heavy chain variable regions of the bispecific antibodies comprise human heavy chain
variable gene segments that are rearranged in vivo within mouse B cells that have been
previously engineered to express a limited human light chain repertoire, or a single human
light chain, cognate with human heavy chains and, in response to exposure with an antigen
of interest, generate a chimeric antibody repertoire containing a plurality of human heavy
chain variable regions that are cognate with one or one of two possible human light chain
variable regions, wherein the chimeric antibodies are specific for the antigen of interest.
In various aspects, there may be a method of preparing a bispecific antibody is
provided, the bispecific antibody comprising 1) a first polypeptide and a second polypeptide,
wherein the first and second polypeptides each include a multimerization domain (e.g., an
immunoglobulin Fc domain) allowing the first and second polypeptides to form a dimer, and
the multimerization domains promote stable interaction between first and second
polypeptides, and wherein one of the multimerization domains bears an amino acid
modification that reduces its affinity to protein A and the other multimerization domain lacks
the modification, 2) a binding domain in each of the first and second polypeptide, each
binding domain comprising a variable heavy chain and a variable light chain, wherein the
variable light chain of the first polypeptide and the variable light chain of the second
polypeptide have a common amino acid sequence, which common sequence has an amino
acid sequence identity to an original light chain of each of the polypeptides of at least 80%,
of at least 85%, preferably at least 90%, more preferably at least 95% and most preferably
100% sequence identity. In various embodiments, the variable light chain is derived from a
human V 1-39 or a human V 3-20 gene segment. In various embodiments, the variable
light chain is a rearranged human light chain sequence. In various embodiments, the
variable light chain is isolated from a mouse as described herein.
In various embodiments, the method comprises the steps of (i) culturing a host
cell comprising a nucleic acid encoding the first polypeptide, the second polypeptide, and the
common light chain, wherein the nucleic acid is expressed; and (ii) recovering the bispecific
antibody from the host cell culture; in one embodiment, the nucleic acid encoding the first
polypeptide or the nucleic acid encoding the second polypeptide, bears an amino acid
modification that reduces its affinity to protein A. In one embodiment, the nucleic acid
encoding the first polypeptide, the second polypeptide, and the common light chain is
present in a single vector or in separate vectors. In one embodiment, the host cell is used to
make a bispecific antibody according to the preceding paragraph.
In one aspect, there may be a method of preparing a bispecific antibody is
provided, comprising (a) selecting a first nucleic acid encoding a first human heavy chain
variable region isolated from a mouse as described herein; (b) selecting a second nucleic
acid encoding a second human heavy chain variable region isolated from the same or
separate mouse as described herein; (c) providing a third nucleic acid encoding a human
light chain variable region isolated from a mouse as described herein or derived from a
rearranged human light chain variable region as described herein; (c) introducing into a host
cell the first, second and third nucleic acids and culturing the host cell so that expression of
the first, second and third nucleic acid occurs; and (d) recovering the bispecific antibody
formed from the cell culture.
In one embodiment, the first and second human heavy chain variable regions are
somatically mutated. In a specific embodiment, the first and second human heavy chain
variable regions are independently derived from a rearranged human V gene segment
selected from 1-2, 1-3, 1-8, 1-18, 1-24, 1-46, 1-58, 1-69, 2-5, 2-26, 2-70, 3-7, 3-9, 3-11, 3-13,
3-15, 3-16, 3-20, 3-21, 3-23, 3-30, 3-33, 3-43, 3-48, 3-53, 3-64, 3-72, 3-73, 4-31, 4-34, 4-39,
4-59, 5-51, and a 6-1 human V gene segment. In one embodiment, the first and second
human heavy chain variable regions are independently derived from a rearranged human V
gene segment selected from 2-5, 3-30 and 3-23. In one embodiment, the first human heavy
chain variable region is derived from a human V 2-5 gene segment and the second human
heavy chain variable region is derived from a human V 3-30 gene segment. In one
embodiment, the first human heavy chain variable region is derived from a human V 3-30
gene segment and the second human heavy chain variable region is derived from a human
V 3-23 gene segment. In one embodiment, the first human heavy chain variable region is
derived from a human V 3-23 gene segment and the second human heavy chain variable
region is derived from a human V 3-30 gene segment.
In one embodiment, the first or second nucleic acid is modified prior to step (c),
wherein the first or second nucleic acid is modified such that it has a reduced affinity to
protein A.
In one embodiment, the third nucleic acid is isolated from a mouse as described
herein. In one embodiment, the third nucleic acid comprises 2 to 5 somatic mutations. In
one embodiment, the third nucleic acid encodes a human light chain variable region derived
from a human V 1-39 gene segment. In one embodiment, the third nucleic acid encodes a
human light chain variable region derived from a human V 3-20 gene segment.
In one embodiment, the third nucleic acid is derived from a rearranged human
light chain variable region. In one embodiment, the rearranged human light chain variable
region comprises a sequence derived from a human V 1-39 gene segment or a human V 3-
gene segment. In one embodiment, the rearranged human light chain variable region
comprises a germline human V 1-39 sequence (i.e., does not comprise a somatic
hypermutation within the V gene segment sequence). In one embodiment, the rearranged
human light chain variable region comprises a germline human V 3-20 sequence.
In various embodiments, a method of preparing a bispecific antibody that
incorporates a first human heavy chain comprising a variable domain derived from a
modified mouse that lacks a rearranged human light chain sequence in its germline is
provided, wherein the first human heavy chain is paired with a cognate human light chain
that comprises a rearranged human light chain variable region derived from a human V 1-39
or a human V 3-20 gene segment. In various embodiments, a second human heavy chain
with a different specificity from the first human heavy chain is identified from an immunized
mouse as described herein. Nucleic acids encoding the two heavy chains and the common
light chain are introduced into a host cell as described in the preceding paragraphs so that
expression of all three chains occurs and the bispecific antibody is recovered from the cell
culture.
In one embodiment, the mouse is immunized with the same antigen used to
generate the first human heavy chain variable domain. In one embodiment, the mouse is
immunized with a different antigen used to generate the first human heavy chain variable
domain.
In one aspect, there may be a method of selecting human heavy chains that can
pair with a single human light chain to make a bispecific antibody is provided, including
nucleic acids that encode the bispecific antibody and a host cell comprising the nucleic
acids.
In one aspect, there may be a method of increasing the amount of a desired
bispecific antibody in a cell culture over undesired products such as monospecific antibodies
is provided, wherein one of the heavy chains of the bispecific antibody is modified to reduce
its affinity to protein A.
In one aspect, there may be an isolated host cell is provided, wherein the host
cell comprises (a) a first nucleic acid sequence encoding a first human heavy chain variable
region that binds a first antigen, wherein the first nucleic acid sequence is isolated from a
mouse immunized with the first antigen that expresses a human immunoglobulin V region
from a rearranged immunoglobulin light chain sequence in the germline of the mouse; (b) a
second nucleic acid sequence encoding a second human heavy chain variable region that
binds a second antigen, wherein the second nucleic acid sequence is isolated from a mouse
immunized with the second antigen that expresses a human immunoglobulin V region from
a rearranged immunoglobulin light chain sequence in the germline of the mouse; (c) a third
nucleic acid sequence encoding a human light chain variable region which, when paired with
the heavy chain variable region of (a) specifically binds the first antigen, and when paired
with the heavy chain variable region of (b) specifically binds to the second antigen.
In various aspects, the first and second antigens are different from one another.
In various aspects, the expression of the first, second and third nucleic acid sequences leads
to the formation of a bispecific antibody that specifically binds to the first and second
antigens.
In one embodiment, the human V region is derived from a rearranged human
light chain sequence comprising a human V 1-39 gene segment or a human V 3-20 gene
segment. In a specific embodiment, the rearranged human light chain sequence is a
germline sequence (i.e., does not comprise a somatic hypermutation within the variable
domain). In one embodiment, the third nucleic acid sequence is isolated from a mouse that
expresses a human immunoglobulin V region from a rearranged immunoglobulin light chain
sequence, wherein the rearranged human light chain sequence is present in the germline of
the mouse. In one embodiment, the rearranged immunoglobulin light chain sequence
comprises a human V 1-39 gene segment or a human V 3-20 gene segment. In a specific
embodiment, the human V 1-39 gene segment or human V 3-20 gene segment comprises
at least one somatic hypermutation in a complementary determining region (CDR) or
framework region (FWR). In a specific embodiment, the first, second and third nucleic acid
sequences are isolated from a mouse that expresses a human immunoglobulin V region
derived from a human V 1-39 or human V 3-20 gene segment from a rearranged
immunoglobulin light chain sequence, wherein the rearranged immunoglobulin light chain
sequence is present in the germline of the mouse.
In various embodiments, the mouse does not contain an endogenous light chain
variable region gene segment that is capable of rearranging to form an immunoglobulin light
chain.
In one embodiment, the human immunoglobulin V region is expressed from a
modified endogenous immunoglobulin light chain locus. In one embodiment, the first and
second antigens are present on one molecule. In one embodiment, the first and second
antigens are present on different molecules. In one embodiment, the first or second nucleic
acid sequence comprises a modification that reduces the affinity of the encoded heavy chain
to protein A.
In one embodiment, the first or second nucleic acid sequences comprise a
rearranged human heavy chain variable region sequence comprising a human heavy chain
gene segment selected from V 1-2, V 1-3, V 1-8, V 1-18, V 1-24, V 1-46, V 1-58, V 1-69,
H H H H H H H H
V 2-5, V 2-26, V 2-70, V 3-7, V 3-9, V 3-11, V 3-13, V 3-15, V 3-20, V 3-21, V 3-23, V 3-
H H H H H H H H H H H H
, V 3-33, V 3-43, V 3-48, V 3-53, V 3-64, V 3-72, V 3-73, V 4-31, V 4-34, V 4-39, V 4-
H H H H H H H H H H H
59, V 5-51, and V 6-1. In a specific embodiment, the heavy chain gene segment is V 2-5,
H H H
V 3-23 or V 3-30.
In one aspect, there may be an antibody or a bispecific antibody comprising a
human heavy chain variable domain made in accordance with the invention is provided. In
another aspect, use of a mouse as described herein to make a fully human antibody or a
fully human bispecific antibody is provided.
In one aspect, there may be a genetically modified mouse, embryo, or cell
described herein comprises a light chain locus that retains endogenous regulatory or
control elements, e.g., a mouse intronic enhancer, a mouse 3’ enhancer, or both an
intronic enhancer and a 3’ enhancer, wherein the regulatory or control elements facilitate
somatic mutation and affinity maturation of an expressed sequence of the light chain locus.
In one aspect, there may be a mouse is provided that comprises a B cell
population characterized by having immunoglobulin light chains derived from no more than
one, or no more than two, rearranged or unrearranged immunoglobulin light chain V and J
gene segments, wherein the mouse exhibits a : light chain ratio that is about the same as
a mouse that comprises a wild type complement of immunoglobulin light chain V and J gene
segments.
In one embodiment, the immunoglobulin light chains are derived from no more
than one, or no more than two, rearranged immunoglobulin light chain V and J gene
segments. In a specific embodiment, the light chains are derived from no more than one
rearranged immunoglobulin light chain V and J gene segments. In one embodiment, the
immunoglobulin light chains are generated from one of two unrearranged immunoglobulin VL
gene segments and one of 1, 2, 3, 4, or 5 immunoglobulin J gene segments. In one
embodiment, the immunoglobulin light chains are generated from one of two unrearranged
immunoglobulin V gene segments and one immunoglobulin J gene segment.
In one aspect, there may be a mouse as described herein is provided that
expresses an immunoglobulin light chain derived from no more than one, or no more than
two, human V /J sequences, wherein the mouse comprises a replacement of all or
substantially all endogenous mouse heavy chain variable region gene segments with one or
more human heavy chain variable region gene segments, and the mouse exhibits a ratio of
(a) CD19 B cells that express an immunoglobulin having a light chain, to (b) CD19 B
cells that express an immunoglobulin having a light chain, of about 1 to about 20.
In one embodiment, the mouse expresses a single light chain derived from a
human V 1-39J 5 sequence, and the ratio of CD19 B cells that express an immunoglobulin
having a light chain to CD19 B cells that express an immunoglobulin having a light chain
is about 1 to about 20; in one embodiment, the ratio is about 1 to at least about 66; in a
specific embodiment, the ratio is about 1 to 66.
In one embodiment, the mouse expresses a single light chain derived from a
human V 3-20J 5 sequence, and the ratio of CD19 B cells that express an immunoglobulin
having a light chain to CD19 B cells that express an immunoglobulin having a light chain
is about 1 to about 20; in one embodiment, the ratio is about 1 to about 21. In specific
embodiments, the ratio is 1 to 20, or 1 to 21.
In some embodiments, the present invention provides a mouse that expresses an
immunoglobulin light chain whose sequence is identical to that achieved by rearrangement
of one of two human V gene segments with 1, 2, 3, 4, or 5 human J gene segments.
In some embodiments, a mouse is provided that expresses an immunoglobulin
light chain generated from a rearrangement of one of two human V gene segments and
one of 1, 2, 3, 4, or 5 human J gene segments, wherein the mouse comprises a
replacement of all or substantially all endogenous immunoglobulin VH gene segments with
one or more human immunoglobulin V , one or more D , and one or more J gene
H H H
segments, and the mouse exhibits a ratio of (a) B cells in the bone marrow that express an
immunoglobulin having a light chain, to (b) B cells in the bone marrow that express an
immunoglobulin having a light chain, of about 1 to about 15. In some embodiments, the
rearrangement includes a human V 1-39 gene segment. In some embodiments, the
rearrangement includes a human V 3-20 gene segment. In some embodiments, the
replacement of the endogenous immunoglobulin V gene segments is at an endogenous
immunoglobulin V locus. In some embodiments, the two human V gene segments is at an
endogenous immunoglobulin V locus, and, in some embodiments, the two human V gene
segments replace all or substantially all mouse immunoglobulin V gene segments. In some
embodiments, the two human V gene segments are at an endogenous immunoglobulin V
locus, and, in some embodiments, the two human V gene segments replace all or
substantially all mouse immunoglobulin V and J gene segments. In various embodiments,
the two human V gene segments are operably linked to two or more (e.g., 2, 3, 4, 5) human
J gene segments.
In some embodiments, a mouse of the present invention expresses a light chain
generated through a rearrangement of a human V 1-39 gene segment or a human V 3-20
gene segment and one of two or more (e.g., 2, 3, 4, or 5) human J gene segments, and the
ratio of immature B cells in the bone marrow that express an immunoglobulin having a light
chain to immature B cells that express an immunoglobulin having a light chain is about 1 to
about 13.
In some embodiments, a mouse of the present invention expresses a light chain
generated through a rearrangement of a human V 1-39 gene segment or a human V 3-20
gene segment and one of two or more (e.g., 2, 3, 4, or 5) human J gene segments, and the
ratio of mature B cells in the bone marrow that express an immunoglobulin having a light
chain to immature B cells that express an immunoglobulin having a light chain is about 1 to
about 7.
In some embodiments, a mouse of the present invention expresses a light chain
generated through a rearrangement of a human V 1-39 gene segment or a human V 3-20
gene segment and one of two or more (e.g., 2, 3, 4, or 5) human J gene segments, and has
a pro B cell population in the bone marrow within in the range of about 2.5x10 to about
4 4 4 4 4
1.5x10 cells, inclusive, for example about 2.5x10 , 3.0x10 , 3.5x10 , 4.0x10 , 4.5x10 ,
4 4 4 4 4 4 4 4 4 4
.0x10 , 5.5x10 , 6.0x10 , 6.5x10 , 7.0x10 , 7.5x10 , 8.0x10 , 8.5x10 , 9.0x10 , 9.5x10 ,
1.0x10 , or 1.5x10 cells; in some embodiments, a mouse of the present invention comprises
a pro B cell population in the bone marrow of about 2.88x10 cells; in some embodiments, a
mouse of the present invention comprises a pro B cell population in the bone marrow of
about 6.42x10 cells; in some embodiments, a mouse of the present invention comprises a
pro B cell population in the bone marrow of about 9.16x10 cells; in some embodiments, a
mouse of the present invention comprises a pro B cell population in the bone marrow of
about 1.19x10 cells. Exemplary pro B cells in the bone marrow of genetically modified mice
as described herein are characterized by expression of CD19, CD43, c-kit and/or a
+ + +
combination thereof (e.g., CD19 , CD43 , c-kit ).
In some embodiments, a mouse of the present invention expresses a light chain
generated through a rearrangement of a human V 1-39 gene segment or a human V 3-20
gene segment and one of two or more (e.g., 2, 3, 4, or 5) human J gene segments, and has
a pre B cell population in the bone marrow within in the range of about 1x10 to about 2x10
6 6 6 6 6 6
cells, inclusive, for example, about 1.0x10 , 1.1x10 , 1.2x10 , 1.3x10 , 1.4x10 , 1.5x10 ,
6 6 6 6 6
1.6x10 , 1.7x10 , 1.8x10 , 1.9x10 , or 2.0x10 cells; in some embodiments, a mouse of the
present invention comprises a pre B cell population in the bone marrow of about 1.25x10
cells; in some embodiments, a mouse of the present invention comprises a pre B cell
population in the bone marrow of about 1.46x10 cells; in some embodiments, a mouse of
the present invention comprises a pre B cell population in the bone marrow of about
1.64x10 cells; in some embodiments, a mouse of the present invention comprises a pre B
cell population in the bone marrow of about 2.03x10 cells. Exemplary pre B cells in the
bone marrow of genetically modified mice as described herein are characterized by
+ - -
expression of CD19, CD43, c-kit and/or a combination thereof (e.g., CD19 , CD43 , c-kit ).
In some embodiments, a mouse of the present invention expresses a light chain
generated through a rearrangement of a human V 1-39 gene segment or a human V 3-20
gene segment and one of two or more (e.g., 2, 3, 4, or 5) human J gene segments, and has
an immature B cell population in the bone marrow within the range of about 5x10 to about
5 5 5
7x10 cells, inclusive, for example, about 5.0x105, 5.1x105, 5.2x10 , 5.3x10 , 5.4x10 ,
5 5 5 5 5 5 5 5 5
.5x10 , 5.6x10 , 5.7x10 , 5.8x10 , 5.9x10 , 6.0x10 , 6.1x10 , 6.2x10 , 6.3x10 , 6.4x10 ,
5 5 5 5 5
6.5x10 , 6.6x10 , 6.7x10 , 6.8x10 , 6.9x10 , or 7.0x10 cells; in some embodiments, a
mouse of the present invention comprises an immature B cell population in the bone marrow
of about 5.33x10 cells; in some embodiments, a mouse of the present invention comprises
an immature B cell population in the bone marrow of about 5.80x10 cells; in some
embodiments, a mouse of the present invention comprises an immature B cell population in
the bone marrow of about 5.92x10 cells; in some embodiments, the mouse comprises an
immature B cell population in the bone marrow of about 6.67x10 cells. Exemplary immature
B cells in the bone marrow of genetically modified mice as described herein are
+ int
characterized by expression of IgM, B220 and/or a combination thereof (e.g., IgM , B220 ).
In some embodiments, a mouse of the present invention expresses a light chain
generated through a rearrangement of a human V 1-39 gene segment or a human V 3-20
gene segment and one of two or more (e.g., 2, 3, 4, or 5) human J gene segments, and has
a mature B cell population in the bone marrow within the range of about 3x10 to about
4 4 4 4 4
1.5x10 cells, inclusive, for example about 3.0x10 , 3.5x10 , 4.0x10 , 4.5x10 , 5.0x10 ,
4 4 4 4 4 4 4 4 4 5
.5x10 , 6.0x10 , 6.5x10 , 7.0x10 , 7.5x10 , 8.0x10 , 8.5x10 , 9.0x10 , 9.5x10 , 1.0x10 , or
1.5x10 cells; in some embodiments, a mouse of the present invention comprises a mature
B cell population in the bone marrow of about 3.11x10 cells; in some embodiments, a
mouse of the present invention comprise a mature B cell population in the bone marrow of
about 1.09x10 cells; in some embodiments, a mouse of the present invention comprises a
mature B cell population in the bone marrow of about 1.16x10 cells; in some embodiments,
a mouse of the present invention comprises a mature B cell population in the bone marrow
of about 1.44x10 cells. Exemplary mature B cells in the bone marrow of genetically
modified mice as described herein are characterized by expression of IgM, B220 and/or a
+ hi
combination thereof (e.g., IgM , B220 ).
In some embodiments, a mouse of the present invention expresses a light chain
generated through a rearrangement of a human V 1-39 gene segment or a human V 3-20
gene segment and one of two or more (e.g., 2, 3, 4, or 5) human J gene segments, and has
a total B cell population in the bone marrow within the range of about 1x10 to about 3x10
6 6 6 6 6 6
cells, inclusive, for example about 1.0x10 , 1.1x10 , 1.2x10 , 1.3x10 , 1.4x10 , 1.5x10 ,
6 6 6 6 6 6 6 6 6 6
1.6x10 , 1.7x10 , 1.8x10 , 1.9x10 , 2.0x10 , 2.1x10 , 2.2x10 , 2.3x10 , 2.4x10 , 2.5x10 ,
6 6 6 6 6
2.6x10 , 2.7x10 , 2.8x10 , 2.9x10 or 2.0x10 cells; in some embodiments, a mouse of the
present invention comprises a total B cell population in the bone marrow of about 1.59x10
cells; in some embodiments, a mouse of the present invention comprises a total B cell
population in the bone marrow of about 1.75x10 cells; in some embodiments, a mouse of
the present invention comprises a total B cell population in the bone marrow of about
2.13x10 cells; in some embodiments, a mouse of the present invention comprises a total B
cell population in the bone marrow of about 2.55x10 cells. An exemplary total B cells in the
bone marrow of genetically modified mice as described herein are characterized by
expression CD19, CD20 and/or a combination thereof (e.g., CD19 ).
In one aspect, there may be a genetically modified mouse is provided that
expresses a single rearranged light chain, wherein the mouse comprises a functional
light chain locus, and wherein the mouse expresses a B cell population that comprises Ig
cells that express a light chain derived from the same single rearranged light chain. In
one embodiment, the percent of Ig Ig B cells in the mouse is about the same as in a wild
type mouse. In a specific embodiment, the percent of Ig Ig B cells in the mouse is about
2 to about 6 percent. In a specific embodiment, the percent of Ig Ig B cells in a mouse
wherein the single rearranged light chain is derived from a V 1-39J 5 sequence is about 2
to about 3; in a specific embodiment, the percent is about 2.6. In a specific embodiment, the
percent of Ig Ig B cells in a mouse wherein the single rearranged light chain is derived
from a V 3-20J 1 sequence is about 4 to about 8; in a specific embodiment, the percent is
about 6.
In some embodiments, a genetically modified mouse is provided that expresses
an immunoglobulin light chain comprising a rearranged human immunoglobulin V /J
sequence, wherein the mouse comprises a functional immunoglobulin light chain locus,
and wherein the mouse comprises a splenic B cell population that comprises a ratio of Ig B
cells to Ig B cells that is about 1 to about 8; in some embodiments, about 1 to about 5. In
some embodiments, the rearranged human immunoglobulin V /J sequence is generated
through a rearrangement of one of two human immunoglobulin V gene segments and one
of 1, 2, 3, 4, or 5 human immunoglobulin J gene segments. In some embodiments, the
rearranged human immunoglobulin V /J sequence is generated through a rearrangement
of a human immunoglobulin V 1-39 gene segment and a human immunoglobulin J gene
segment selected from J 1, J 2, J 3, J 4, J 5, and a combination thereof. In some
embodiments, the rearranged human immunoglobulin V /J sequence is generated through
a rearrangement of a human immunoglobulin V 3-20 gene segment and a human
immunoglobulin J gene segment selected from J 1, J 2, J 3, J 4, J 5, and a combination
thereof.
In some embodiments, a mouse of the present invention comprises a CD19
splenic B cell population within the range of about 2x10 to about 7x10 cells, inclusive, for
6 6 6 6 6 6 6 6
example about 2.0x10 , 2.5x10 , 3.0x10 , 3.5x10 , 4.0x10 , 4.5x10 , 5.0x10 , 5.5x10 ,
6 6 6
6.0x10 , 6.5x10 , or 7.0x10 cells; in some embodiments, a mouse of the present invention
comprises a CD19 splenic B cell population of about 2.74x10 cells; some embodiments, a
mouse of the present invention comprises a CD19 splenic B cell population of about
4.30x10 cells; in some embodiments, a mouse of the present invention comprises a CD19
splenic B cell population of about 5.53x10 cells; in some embodiments, a mouse of the
present invention comprises a CD19 splenic B cell population of about 6.18x10 cells.
In some embodiments, a mouse of the present invention comprises a CD19 ,
hi lo 6 6
IgD , IgM splenic B cell population within the range of about 1x10 to about 4x10 cells,
6 6 6 6 6 6 6
inclusive, for example about 1.0x10 , 1.5x10 , 2.0x10 , 2.5x10 , 3.0x10 , 3.5x10 , 4.0x10
+ hi
cells; in some embodiments, a mouse of the present invention comprises a CD19 , IgD ,
lo 6
IgM splenic B cell population of about 1.30x10 ; in some embodiments, a mouse of the
+ hi lo 6
present invention comprises a CD19 , IgD , IgM splenic B cell population of about 2.13x10
+ hi lo
cells; in some embodiments, a mouse of the present invention comprises CD19 , IgD , IgM
splenic B cell population of about 3.15x10 cells; in some embodiments, a mouse of the
+ hi lo 6
present invention comprises a CD19 , IgD , IgM splenic B cell population of about 3.93x10
cells.
In some embodiment, a mouse of the present invention comprises a CD19 ,
lo hi 5 6
IgD , IgM splenic B cell population within the range of about 9x10 to about 2x10 cells,
5 5 5 6 6
inclusive, for example about 9.0x10 , 9.25x10 , 9.5x10 , 9.75x10 , 1.0x10 , 1.25x10 ,
6 6 6
1.50x10 , 1.75x10 , 2.0x10 cells; in some embodiments, a mouse of the present invention
+ lo hi 5
comprises a CD19 , IgD , IgM splenic B cell population of about 9.52x10 ; in some
+ lo hi
embodiments, a mouse of the present invention comprises a CD19 , IgD , IgM splenic B
cell population of about 1.23x10 cells; in some embodiments, a mouse of the present
+ lo hi 6
invention comprises CD19 , IgD , IgM splenic B cell population of about 1.40x10 cells; in
+ lo hi
some embodiments, a mouse of the present invention comprises a CD19 , IgD , IgM
splenic B cell population of about 1.42x10 cells.
In some embodiments, a genetically modified mouse is provided, wherein the
mouse comprises an immunoglobulin light chain locus that comprises two unrearranged
human immunoglobulin V gene segments and two or more (e.g., 2, 3, 4, or 5) unrearranged
human J gene segments, and wherein the mouse comprises a peripheral splenic B cell
population comprising transitional (e.g., T1, T2 and T3) B cell populations that are about the
same as a mouse that comprises a wild type complement of immunoglobulin light chain V
and J gene segments. Exemplary transitional B cell populations (e.g., T1, T2 and T3) in the
spleen of a genetically modified mouse as described herein are characterized by expression
of IgM, CD23, CD93, B220 and/or a combination thereof.
In some embodiments, a mouse of the present invention comprises a T1 B cell
+ + hi - 6
population in the spleen (e.g., CD93 , B220 , IgM , CD23 ) within the range of about 2x10
6 6 6 6 6
to about 7x10 cells, inclusive, for example about 2.0x10 , 2.5x10 , 3.0x10 , 3.5x10 ,
6 6 6 6 6 6 6
4.0x10 , 4.5x10 , 5.0x10 , 5.5x10 , 6.0x10 , 6.5x10 , or 7.0x10 cells; in some embodiments,
a mouse of the present invention comprises a T1 B cell population in the spleen of about
2.16x10 cells; in some embodiments, a mouse of the present invention comprises a T1 B
cell population in the spleen of about 3.63x10 cells; in some embodiments, a mouse of the
present invention comprises a T1 B cell population in the spleen of about 3.91x10 ; in some
embodiments, a mouse of the present invention comprises a T1 B cell population in the
spleen of about 6.83x10 cells.
In some embodiments, a mouse of the present invention comprises a T2 B cell
+ + hi + 6
population in the spleen (e.g., CD93 , B220 , IgM , CD23 ) within the range of about 1x10
6 6 6 6 6
to about 7x10 cells, inclusive, for example about 1.0x10 , 1.5x10 , 2.0x10 , 2.5x10 ,
6 6 6 6 6 6 6 6 6
3.0x10 , 3.5x10 , 4.0x10 , 4.5x10 , 5.0x10 , 5.5x10 , 6.0x10 , 6.5x10 , or 7.0x10 cells; in
some embodiments, a mouse of the present invention mouse comprises a T2 B cell
population in the spleen of about 1.30x10 cells; in some embodiments, a mouse of the
present invention comprises a T2 B cell population in the spleen of about 2.46x10 cells; in
some embodiments, a mouse of the present invention comprises a T2 B cell population in
the spleen of about 3.24x10 ; in some embodiments, a mouse of the present invention
comprises a T2 B cell population in the spleen of about 6.52x10 cells.
In some embodiments, a mouse of the present invention comprises a T3 B cell
+ + lo + 6
population in the spleen (e.g., CD93 , B220 , IgM , CD23 ) within the range of about 1x10
6 6 6 6 6
to about 4x10 cells, inclusive, for example about 1.0x10 , 1.5x10 , 2.0x10 , 2.5x10 ,
6 6 6
3.0x10 , 3.5x10 , or 4.0x10 cells; in some embodiments, a mouse of the present invention
comprises a T3 B cell population in the spleen of about 1.08x10 cells; in some
embodiments, a mouse of the present invention comprises a T3 B cell population in the
spleen of about 1.35x10 cells; in some embodiments, a mouse of the present invention
comprises a T3 B cell population in the spleen of about 3.37x10 ; in some embodiments, a
mouse of the present invention comprises a T1 B cell population in the spleen of about
3.63x10 cells.
In some embodiments, a genetically modified mouse is provided, wherein the
mouse comprises an immunoglobulin light chain locus that comprises two unrearranged
human immunoglobulin V gene segments and 1, 2, 3, 4, or 5 unrearranged human
immunoglobulin J gene segments, and wherein the mouse comprises a peripheral splenic
B cell population comprising marginal zone and marginal zone precursor B cell populations
that are about the same as a mouse that comprises a wild type complement of
immunoglobulin V and J gene segments. Exemplary marginal zone B cell populations in
the spleen of a genetically modified mouse as described herein are characterized by
expression of IgM, CD21/35, CD23, CD93, B220 and/or a combination thereof.
In some embodiments, a mouse of the present invention comprises marginal
- + hi hi -
zone B cell population in the spleen (e.g., CD93 , B220 , IgM , CD21/35 , CD23 ) within the
6 6 6 6
range of about 1x10 to about 3x10 cells, inclusive, for example, about 1.0x10 , 1.5x10 ,
6 6 6
2.0x10 , 2.5x10 , or 3.0x10 cells; in some embodiments, a mouse of the present invention
comprises a marginal zone B cell population in the spleen of about 1.47x10 cells; in some
embodiments, a mouse of the present invention comprises a marginal zone B cell population
in the spleen of about 1.49x10 cells; in some embodiments, a mouse of the present
invention comprises a marginal zone B cell population in the spleen of about 2.26x10 cells;
in some embodiments, a mouse of the present invention comprises a marginal zone B cell
population in the spleen of about 2.33x10 cells.
In some embodiments, a genetically modified mouse is provided, wherein the
mouse comprises an immunoglobulin light chain locus that comprises two unrearranged
human immunoglobulin V gene segments and 1, 2, 3, 4, or 5 unrearranged human
immunoglobulin J gene segments, and wherein the mouse comprises a peripheral splenic
B cell population comprising follicular (e.g., FO-I and FO-II) B cell population(s) that are
about the same as a mouse that comprises a wild type complement of immunoglobulin V
and J gene segments. Exemplary follicular B cell populations (e.g., FO-I and FO-II) in the
spleen of a genetically modified mouse as described herein are characterized by expression
of IgM, IgD, CD21/35, CD93, B220 and/or a combination thereof.
In some embodiments, a mouse of the present invention comprises a follicular
- + int lo hi
type 1 B cell population in the spleen (e.g., CD93 , B220 , CD21/35 , IgM , IgD ) within the
6 7 6 6
range of about 3x10 to about 1.5x10 cells, inclusive, for example about 3.0x10 , 3.5x10 ,
6 6 6 6 6 6 6 6 6 6
4.0x10 , 4.5x10 , 5.0x10 , 5.5x10 , 6.0x10 , 6.5x10 , 7.0x10 , 7.5x10 , 8.0x10 , 8.5x10 ,
6 6 7 7
9.0x10 , 9.5x10 , 1.0x10 , or 1.5x10 cells; in some embodiments, a mouse of the present
invention comprises a follicular type 1 B cell population in the spleen of about 3.57x10 cells;
in some embodiments, a mouse of the present invention comprises a follicular type 1 B cell
population in the spleen of about 6.31x10 cells; in some embodiments, a mouse of the
present invention comprises a follicular type 1 B cell population in the spleen of about
9.42x10 cells; in some embodiments, a mouse of the present invention comprise a follicular
type 1 B cell population in the spleen of about 1.14x10 cells.
In some embodiments, a mouse of the present invention comprises a follicular
- + int int hi
type 2 B cell population in the spleen (e.g., CD93 , B220 , CD21/35 , IgM , IgD ) within the
6 6 6 6 6
range of about 1x10 to about 2x10 cells, inclusive, for example, 1.0x10 , 1.25x10 , 1.5x10 ,
1.75x10 , or 2.0x10 cells; in some embodiments, a mouse of the present invention
comprises a follicular type 2 B cell population in the spleen of about 1.14x10 cells; in some
embodiments, a mouse of the present invention comprises a follicular type 2 B cell
population in the spleen of about 1.45x10 cells; in some embodiments, a mouse of the
present invention comprises a follicular type 2 B cell population in the spleen of about
1.80x10 ; in some embodiments, a mouse of the present invention comprise a follicular type
2 B cell population in the spleen of about 2.06x10 cells.
In one aspect, there may be a genetically modified mouse is provided, wherein
the mouse expresses a single rearranged light chain derived from a human V and J
gene segment, wherein the mouse expresses a B cell population that comprises a single
light chain derived from the single rearranged light chain sequence, wherein the genetically
modified mouse has not been rendered resistant to somatic hypermutations. In one
embodiment, at least 90% of the light chains expressed on a B cell of the mouse exhibit
from at least one to about five somatic hypermutations.
In one aspect, there may be a genetically modified mouse is provided that is
modified to express a single light chain derived from no more than one, or no more than
two, rearranged light chain sequences, wherein the mouse exhibits a light chain usage
that is about two-fold or more, at least about three-fold or more, or at least about four-fold or
more greater than the light chain usage exhibited by a wild type mouse, or greater than the
light chain usage exhibited by a mouse of the same strain that comprises a wild type
repertoire of light chain gene segments. In a specific embodiment, the mouse expresses
the single light chain from no more than one rearranged light chain sequence. In a more
specific embodiment, the rearranged light chain sequence is selected from a V 1-39J 5
and V 3-20J 1 sequence. In one embodiment, the rearranged light chain sequence is a
V 1-39J 5 sequence. In one embodiment, the rearranged light chain sequence is a V 3-
20J 1 sequence.
In one aspect, there may be a genetically modified mouse is provided that
expresses a single light chain derived from no more than one, or no more than two,
rearranged light chain sequences, wherein the mouse exhibits a light chain usage that is
about 100-fold or more, at least about 200-fold or more, at least about 300-fold or more, at
least about 400-fold or more, at least about 500-fold or more, at least about 600-fold or
more, at least about 700-fold or more, at least about 800-fold or more, at least about 900-
fold or more, at least about 1000-fold or more greater than the same light chain usage
exhibited by a mouse bearing a complete or substantially complete human light chain
locus. In a specific embodiment, the mouse bearing a complete or substantially complete
human light chain locus lacks a functional unrearranged mouse light chain sequence. In
a specific embodiment, the mouse expresses the single light chain from no more than one
rearranged light chain sequence. In one embodiment, the mouse comprises one copy of a
rearranged light chain sequence (e.g., a heterozygote). In one embodiment, the mouse
comprises two copies of a rearranged light chain sequence (e.g., a homozygote). In a
more specific embodiment, the rearranged light chain sequence is selected from a V 1-
39J 5 and V 3-20J 1 sequence. In one embodiment, the rearranged light chain
sequence is a V 1-39J 5 sequence. In one embodiment, the rearranged light chain
sequence is a V 3-20J 1 sequence.
In one aspect, there may be a genetically modified mouse is provided that
expresses a single light chain derived from no more than one, or no more than two,
rearranged light chain sequences, wherein the light chain in the genetically modified mouse
exhibits a level of expression that is at least 10-fold to about 1,000-fold, 100-fold to about
1,000-fold, 200-fold to about 1,000-fold, 300-fold to about 1,000-fold, 400-fold to about
1,000-fold, 500-fold to about 1,000-fold, 600-fold to about 1,000-fold, 700-fold to about
1,000-fold, 800-fold to about 1,000-fold, or 900-fold to about 1,000-fold higher than
expression of the same rearranged light chain exhibited by a mouse bearing a complete or
substantially complete light chain locus. In one embodiment, the light chain comprises a
human sequence. In a specific embodiment, the human sequence is a sequence. In one
embodiment, the human sequence is a sequence. In one embodiment, the light chain is a
fully human light chain.
In one embodiment, the level of expression is characterized by quantitating
mRNA of transcribed light chain sequence, and comparing it to transcribed light chain
sequence of a mouse bearing a complete or substantially complete light chain locus.
In one aspect, there may be a genetically modified mouse is provided that
expresses a single light chain derived from no more than one, or no more than two,
rearranged light chain sequences, wherein the mouse, upon immunization with antigen,
exhibits a serum titer that is comparable to a wild type mouse immunized with the same
antigen. In a specific embodiment, the mouse expresses a single light chain from no more
than one rearranged light chain sequence. In one embodiment, the serum titer is
characterized as total immunoglobulin. In a specific embodiment, the serum titer is
characterized as IgM specific titer. In a specific embodiment, the serum titer is characterized
as IgG specific titer. In a more specific embodiment, the rearranged light chain sequence
is selected from a V 1-39J 5 and V 3-20J 1 sequence. In one embodiment, the
rearranged light chain sequence is a V 1-39J 5 sequence. In one embodiment, the
rearranged light chain sequence is a V 3-20J 1 sequence.
In one aspect, there may be a genetically modified mouse is provided that
expresses a population of antigen-specific antibodies, wherein all of the immunoglobulin light
chains of the population of antigen-specific antibodies comprise a human light chain variable
(V ) region derived from the same single human V gene segment and the immunoglobulin
heavy chains comprise a human heavy chain variable (V ) region derived from one of a
plurality of human V gene segments.
In various embodiments, the human V gene segments are selected from V 1-2,
V 1-3, V 1-8, V 1-18, V 1-24, V 1-46, V 1-58, V 1-69, V 2-5, V 2-26, V 2-70, V 3-7, V 3-
H H H H H H H H H H H H
9, V 3-11, V 3-13, V 3-15, V 3-20, V 3-21, V 3-23, V 3-30, V 3-33, V 3-43, V 3-48, V 3-
H H H H H H H H H H H
53, V 3-64, V 3-72, V 3-73, V 4-31, V 4-34, V 4-39, V 4-59, V 5-51, and V 6-1.
H H H H H H H H H
In various embodiments, same single human V gene segment is selected from a
human V 1-39 gene segment and a human V 3-20 gene segment. In various
embodiments, all of the immunoglobulin light chains comprise a human light chain J (J )
gene segment selected from a J and a J gene segment. In a specific embodiment, the
human J gene segment is selected from a human J 1 and a J 5 gene segment. In various
embodiments, the mouse lacks a sequence selected from a mouse immunoglobulin V gene
segment, a mouse immunoglobulin J gene segment, and a combination thereof. In various
embodiments, the human V region is operably linked to a human, mouse, or rat
immunoglobulin light chain constant (C ) region. In a specific embodiment, the human V
region is operably linked to a mouse C region. In a specific embodiment, the human V
region is operably linked to a rat C region.
In various embodiments, the human V region is expressed from an endogenous
immunoglobulin light chain locus. In various embodiments, the human V region is operably
linked to a human, mouse, or rat immunoglobulin heavy chain constant (C ) region. In
various embodiments the (C ) region comprises a human sequence selected from a C 1, a
hinge, a C 2, a C 3, a C 4, and/or a combination thereof. In various embodiments, the
H H H
human VH region is expressed from an endogenous immunoglobulin heavy chain locus.
In one aspect, there may be a genetically modified mouse is provided that
expresses a plurality of immunoglobulin heavy chains associated with a single light chain. In
one embodiment, the heavy chain comprises a human sequence. In various embodiments,
the human sequence is selected from a variable sequence, a C 1, a hinge, a C 2, a C 3,
H H H
and a combination thereof. In one embodiment, the single light chain comprises a human
sequence. In various embodiments, the human sequence is selected from a variable
sequence, a constant sequence, and a combination thereof. In one embodiment, the mouse
comprises a disabled endogenous immunoglobulin locus and expresses the heavy chain
and/or the light chain from a transgene or extrachromosomal episome. In one embodiment,
the mouse comprises a replacement at an endogenous mouse locus of some or all
endogenous mouse heavy chain gene segments (i.e., V, D, J), and/or some or all
endogenous mouse heavy chain constant sequences (e.g., C 1, hinge, C 2, C 3, or a
H H H
combination thereof), and/or some or all endogenous mouse light chain sequences (e.g., V,
J, constant, or a combination thereof), with one or more human immunoglobulin sequences.
In one aspect, there may be a mouse suitable for making antibodies that have the
same light chain is provided, wherein all or substantially all antibodies made in the mouse
are expressed with the same light chain. In one embodiment, the light chain is expressed
from an endogenous light chain locus.
In one aspect, there may be a method for making a light chain for a human
antibody is provided, comprising obtaining from a mouse as described herein a light chain
sequence and a heavy chain sequence, and employing the light chain sequence and the
heavy chain sequence in making a human antibody. In one embodiment, the human
antibody is a bispecific antibody.
In one aspect, there may be a method for identifying a human heavy chain
variable domain that is capable of binding an antigen of interest with an engineered light
chain as described herein is provided, wherein the method comprises providing a heavy
chain variable domain derived from a first antibody that is capable of binding the antigen,
repairing the heavy chain variable domain with a germline light chain sequence and
transfecting a cell so that each are expressed to form a second antibody, exposing the
second antibody to the antigen, and measuring binding of the second antibody to the
antigen.
In one embodiment, the light chain of the first antibody comprises a human V 1-
39 sequence. In one embodiment, the light chain of the first antibody comprises a human
V 3-20 sequence. In one embodiment, the germline light chain sequence comprises a
human V 1-39 or V 3-20 sequence. In various embodiments, binding of the second
antibody to the antigen is determined by comparison of binding of the first antibody to the
antigen.
Any of the embodiments and aspects described herein can be used in
conjunction with one another, unless otherwise indicated or apparent from the context.
Other embodiments will become apparent to those skilled in the art from a review of the
ensuing description.
BRIEF DESCRIPTION OF FIGURES
illustrates a targeting strategy for replacing endogenous mouse
immunoglobulin light chain variable region gene segments with a human V 1-39J 5 gene
region.
illustrates a targeting strategy for replacing endogenous mouse
immunoglobulin light chain variable region gene segments with a human V 3-20J 1 gene
region.
illustrates a targeting strategy for replacing endogenous mouse
immunoglobulin light chain variable region gene segments with a human VpreB/J 5 gene
region.
shows the percent of CD19 B cells (y-axis) from peripheral blood for wild
type mice (WT), mice homozygous for an engineered human rearranged V 1-39J 5 light
chain region (V 1-39J 5 HO) and mice homozygous for an engineered human rearranged
V 3-20J 1 light chain region (V 3-20J 1 HO).
shows the relative mRNA expression (y-axis) of a V 1derived light
chain in a quantitative PCR assay using probes specific for the junction of an engineered
human rearranged V 1-39J 5 light chain region (V 1-39J 5 Junction Probe) and the human
V 1-39 gene segment (V 1-39 Probe) in a mouse homozygous for a replacement of the
endogenous V and J gene segments with human V and J gene segments (H ), a wild
type mouse (WT), and a mouse heterozygous for an engineered human rearranged V 1-
39J 5 light chain region (V 1-39J 5 HET). Signals are normalized to expression of mouse
C . N.D.: not detected.
shows the relative mRNA expression (y-axis) of a V 1derived light
chain in a quantitative PCR assay using probes specific for the junction of an engineered
human rearranged V 1-39J 5 light chain region (V 1-39J 5 Junction Probe) and the human
V 1-39 gene segment (V 1-39 Probe) in a mouse homozygous for a replacement of the
endogenous V and J gene segments with human V and J gene segments (H ), a wild
type mouse (WT), and a mouse homozygous for an engineered human rearranged V 1-
39J 5 light chain region (V 1-39J 5 HO). Signals are normalized to expression of mouse
C .
shows the relative mRNA expression (y-axis) of a V 3derived light
chain in a quantitative PCR assay using probes specific for the junction of an engineered
human rearranged V 3-20J1 light chain region (V 3-20J 1 Junction Probe) and the human
V 3-20 gene segment (V 3-20 Probe) in a mouse homozygous for a replacement of the
endogenous V and J gene segments with human V and J gene segments (H ), a wild
type mouse (WT), and a mouse heterozygous (HET) and homozygous (HO) for an
engineered human rearranged V 3-20J1 light chain region. Signals are normalized to
expression of mouse C .
shows IgM (left) and IgG (right) titer in wild type (WT; N=2) and mice
homozygous for an engineered human rearranged V 1-39J 5 light chain region (V 1-39J 5
HO; N=2) immunized with -galatosidase.
shows total immunoglobulin (IgM, IgG, IgA) titer in wild type (WT; N=5)
and mice homozygous for an engineered human rearranged V 3-20J 1 light chain region
(V 3-20J 1 HO; N=5) immunized with -galatosidase.
shows a schematic of monospecific antibodies (Parent-1 and Parent-2)
and a bispecific antibody (Bispecific) constructed from heavy chain variable regions from
each parent monospecific antibody. A common light chain variable region (darkened) is
indicated in the bispecific antibody.
shows a schematic for the binding characteristics of two parent
monoclonal antibodies (Parent-1 and Parent-2) for an antigen of interest, as well as the
binding characteristic of a bispecific antibody constructed from pairing the heavy chain
variable regions from each monospecific parent antibody with a common light chain. The
capability of the bispecific antibody to bind to two distinct epitopes of the antigen of interest
either separately (bottom left) or simultaneously (bottom right) is indicated.
shows a bar graph of the binding of 300nM bispecific (darkened bars) and
monospecific (striped and gray bars) antibodies to a captured monomeric Antigen E surface
in BIACORE™ units (RU). Monoclonal parent-1 antibody (P1 Ab), monoclonal parent-2 (P2
Ab) and bispecific antibodies (BsAb) are indicated.
shows two genetically modified endogenous immunoglobulin light chain
(e.g., light chain) loci. The locus on the top (DLC-5J) contains an engineered human DNA
fragment (striped line) containing two human V gene segments and five human J gene
segments. The locus on the bottom (DLC-1J) contains an engineered human DNA fragment
(striped line) containing two human V gene segments and one human J gene segment.
Each locus is capable of rearranging to form a human V region operably linked to an
endogenous light chain constant region (e.g., a C ). Immunoglobulin promoters (arrow
above locus), leader exons (closed arrows), and the two human V gene segments (open
arrows), all flanked upstream (5’) by a neomycin cassette containing Frt recombination sites
are shown. Recombination signal sequences engineered with each of the human gene
segments (V and J ) are indicated by open ovals juxtaposed with each gene segment.
A, in the top panel, shows representative contour plots of bone marrow
stained for B and T cells (CD19 and CD3 , respectively) from a wild type mouse (WT) and a
mouse homozygous for two human V and five human J gene segments (DLC-5J). The
bottom panel shows representative contour plots of bone marrow gated on CD19 and
stained for ckit and CD43 from a wild type mouse (WT) and a mouse homozygous for two
human V and five human J gene segments (DLC-5J). Pro and Pre B cells are noted on
the contour plots of the bottom panel.
+ + + + –
B shows the number of Pro (CD19 CD43 ckit ) and Pre (CD19 CD43
ckit ) B cells in bone marrow harvested from the femurs of wild type mice (WT) and mice
homozygous for two human V and five human J gene segments (DLC-5J).
A shows representative contour plots of bone marrow gated on singlets
stained for immunoglobulin M (IgM) and B220 from a wild type mouse (WT) and a mouse
homozygous for two human V and five human J gene segments (DLC-5J). Immature,
mature and pro/pre B cells are noted on each of the contour plots.
+ int +
B shows the total number of B (CD19 ), immature B (B220 IgM ) and
hi +
mature B (B220 IgM ) cells in bone marrow isolated from the femurs of wild type mice (WT)
and mice homozygous for two human V and five human J gene segments (DLC-5J).
A shows representative contour plots of bone marrow gated on singlets
stained for immunoglobulin M (IgM) and B220 from a wild type mouse (WT) and a mouse
homozygous for two human V and five human J gene segments (DLC-5J). Immature,
mature and pro/pre B cells are noted on each of the contour plots.
B shows representative contour plots of bone marrow gated on immature
int + hi +
(B220 IgM ) and mature (B220 IgM ) B cells stained for Ig and Ig expression isolated
from the femurs of a wild type mouse (WT) and a mouse homozygous for two human V and
five human J gene segments (DLC-5J).
A, in the top panel, shows representative contour plots of splenocytes
gated on singlets and stained for B and T cells (CD19 and CD3 , respectively) from a wild
type mouse (WT) and a mouse homozygous for two human V and five human J gene
segments (DLC-5J). The bottom panel shows representative contour plots of splenocytes
gated on CD19 and stained for immunoglobulin D (IgD) and immunoglobulin M (IgM) from a
wild type mouse (WT) and a mouse homozygous for two human V and five human J gene
segments (DLC-5J). Mature (54 for WT, 56.9 for DLC-5J) and transitional (23.6 for WT, 25.6
for DLC-5J) B cells are noted on each of the contour plots.
B shows the total number of CD19 B cells, transitional B cells
+ hi lo + lo hi
(CD19 IgM IgD ) and mature B cells (CD19 IgM IgD ) in harvested spleens from wild type
mice (WT) and mice homozygous for two human V and five human J gene segments
(DLC-5J).
A shows representative contour plots of Ig and Ig splenocytes gated
on CD19 from a wild type mouse (WT) and a mouse homozygous for two human V and
five human J gene segments (DLC-5J).
+ + + +
B shows the total number of B cells (CD19 ), Ig B cells (CD19 Ig ) and
+ + +
Ig B cells (CD19 Ig ) in harvested spleens from wild type (WT) and mice homozygous for
two human V and five human J gene segments (DLC-5J).
A shows the peripheral B cell development in mice homozygous for two
human V and five human J gene segments. The first (far left) contour plot shows CD93
and B220 splenocytes gated on CD19 indicating immature (39.6) and mature (57.8) B
cells. The second (top middle) contour plot shows IgM and CD23 expression in immature
- + lo - hi hi mid +
B cells indicating T1 (33.7; IgD IgM CD21 CD23 ), T2 (21.2; IgD IgM CD21 CD23 ) and
T3 (29.1) B cell populations. The third (bottom middle) contour plot shows CD21 (CD35 )
and IgM expression of mature B cells indicating a small population (14.8) which give rise to
marginal zone B cells and a second population (70.5) which gives rise to follicular (FO) B
cells. The fourth (top right) contour plot shows B220 and CD23 expression in mature B
cells indicating marginal zone (90.5; MZ) and marginal zone precursor (7.3;
hi hi hi + +
IgM IgD CD21 CD23 ) B cell populations. The fifth (bottom right) contour plot shows IgD
+ hi lo mid +
and IgM expression in mature B cells indicating FO-I (79.0; IgD IgM CD21 CD23 ) and
hi hi mid +
FO-II (15.1; IgD IgM CD21 CD23 ) B cell populations. Percentage of cells within each
gated region is shown.
B shows the peripheral B cell development in wild type mice. The first
+ + +
(far left) contour plot shows CD93 and B220 splenocytes gated on CD19 indicating
immature (31.1) and mature (64.4) B cells. The second (top middle) contour plot shows
+ + - + lo -
IgM and CD23 expression in immature B cells indicating T1 (28.5; IgD IgM CD21 CD23 ),
hi hi mid +
T2 (28.7; IgD IgM CD21 CD23 ) and T3 (30.7) B cell populations. The third (bottom
+ + +
middle) contour plot shows CD21 (CD35 ) and IgM expression of mature B cells indicating
a small population (7.69) which give rise to marginal zone B cells and a second population
(78.5) which gives rise to follicular (FO) B cells. The fourth (top right) contour plot shows
B220 and CD23 expression in mature B cells indicating marginal zone (79.9; MZ) and
hi hi hi +
marginal zone precursor (19.4; IgM IgD CD21 CD23 ) B cell populations. The fifth (bottom
right) contour plot shows IgD and IgM expression in mature B cells indicating FO-I (83.6;
hi lo mid + hi hi mid +
IgD IgM CD21 CD23 ) and FO-II (13.1; IgD IgM CD21 CD23 ) B cell populations.
Percentage of cells within each gated region is shown.
shows the total number of transitional, marginal zone and follicular B cell
populations in harvested spleens of wild-type (WT) and mice homozygous for two human V
and five human J gene segments (DLC-5J).
shows the relative mRNA expression in bone marrow (y-axis) of V 3
derived and V 1derived light chains in a quantitative PCR assay using probes specific
for V 3-20 or V 1-39 gene segments in mice homozygous for a replacement of the
endogenous V and J gene segments with human V and J gene segments (H ), wild
type mice (WT), mice homozygous for two human V gene segments and five human J
gene segments (DLC-5J) and mice homozygous for two human V gene segments and one
human J gene segment (DLC-1J). Signals are normalized to expression of mouse C .
ND: not detected.
shows the relative mRNA expression in whole spleens (y-axis) of V 3
derived and V 1derived light chains in a quantitative PCR assay using probes specific
for V 3-20 or V 1-39 gene segments in mice homozygous for a replacement of the
endogenous V and J gene segments with human V and J gene segments (H ), wild
type mice (WT), mice homozygous for two human V gene segments and five human J
gene segments (DLC-5J) and mice homozygous for two human V gene segments and one
human J gene segment (DLC-1J). Signals are normalized to expression of mouse C .
ND: not detected.
shows a general illustration of recombination of a V and a J gene
segment of an immunoglobulin light chain allele in a mouse and the structure of the light
chain locus before rearrangement (top) and after rearrangement (bottom). Such a
rearrangement as shown is only one of several possible rearrangement events.
DETAILED DESCRIPTION
This invention is not limited to particular methods, and experimental conditions
described, as such methods and conditions may vary. It is also to be understood that the
terminology used herein is for the purpose of describing particular embodiments only, and is
not intended to be limiting, since the scope of the present invention is defined by the claims.
Unless defined otherwise, all terms and phrases used herein include the
meanings that the terms and phrases have attained in the art, unless the contrary is clearly
indicated or clearly apparent from the context in which the term or phrase is used. Although
any methods and materials similar or equivalent to those described herein can be used in
the practice or testing of the present invention, particular methods and materials are now
described. All publications mentioned are hereby incorporated by reference in their entirety.
The term "antibody", as used herein, includes immunoglobulin molecules
comprising four polypeptide chains, two heavy (H) chains and two light (L) chains inter-
connected by disulfide bonds. Each heavy chain comprises a heavy chain variable (V )
region and a heavy chain constant region (C ). The heavy chain constant region comprises
three domains, C 1, C 2 and C 3. Each light chain comprises a light chain variable (V )
H H H L
region and a light chain constant region (C ). The V and V regions can be further
L H L
subdivided into regions of hypervariability, termed complementarity determining regions
(CDR), interspersed with regions that are more conserved, termed framework regions (FR).
Each V and V comprises three CDRs and four FRs, arranged from amino-terminus to
carboxy-terminus in the following order: FR1, CDR1, FR2, CDR2, FR3, CDR3, FR4 (heavy
chain CDRs may be abbreviated as HCDR1, HCDR2 and HCDR3; light chain CDRs may be
abbreviated as LCDR1, LCDR2 and LCDR3. The term “high affinity” antibody refers to an
antibody that has a K with respect to its target epitope about of 10 M or lower (e.g., about
-9 -10 -11 -12
1 x 10 M, 1 x 10 M, 1 x 10 M, or about 1 x 10 M). In one embodiment, K is
measured by surface plasmon resonance, e.g., BIACORE™; in another embodiment, K is
measured by ELISA.
The phrase “bispecific antibody” refers to an antibody capable of selectively
binding two or more epitopes. Bispecific antibodies include fragments of two different
monoclonal antibodies () and generally comprise two nonidentical heavy chains
derived from the two different monoclonal antibodies, with each heavy chain specifically
binding a different epitope—either on two different molecules (e.g., different epitopes on two
different immunogens; see , bottom left) or on the same molecule (e.g., different
epitopes on the same immunogen; see , bottom right). If a bispecific antibody is
capable of selectively binding two different epitopes (a first epitope and a second epitope),
the affinity of the first heavy chain for the first epitope will generally be at least one to two or
three or four or more orders of magnitude lower than the affinity of the first heavy chain for
the second epitope, and vice versa. Epitopes specifically bound by the bispecific antibody
can be on the same or a different target (e.g., on the same or a different protein; see ). Exemplary bispecific antibodies include those with a first heavy chain specific for a
tumor antigen and a second heavy chain specific for a cytotoxic marker, e.g., an Fc receptor
(e.g., Fc RI, Fc RII, Fc RIII, etc.) or a T cell marker (e.g., CD3, CD28, etc.). Further, the
second heavy chain variable region can be substituted with a heavy chain variable region
having a different desired specificity. For example, a bispecific antibody with a first heavy
chain specific for a tumor antigen and a second heavy chain specific for a toxin can be
paired so as to deliver a toxin (e.g., saporin, vinca alkaloid, etc.) to a tumor cell. Other
exemplary bispecific antibodies include those with a first heavy chain specific for an
activating receptor (e.g., B cell receptor, Fc RI, Fc RIIA, Fc RIIIA, Fc RI, T cell receptor,
etc.) and a second heavy chain specific for an inhibitory receptor (e.g., Fc RIIB, CD5, CD22,
CD72, CD300a, etc.). Such bispecific antibodies can be constructed for therapeutic
conditions associated with cell activation (e.g. allergy and asthma). Bispecific antibodies can
be made, for example, by combining heavy chains that recognize different epitopes of the
same or different immunogen (). For example, nucleic acid sequences encoding
heavy chain variable sequences that recognize different epitopes of the same or different
immunogen can be fused to nucleic acid sequences encoding the same or different heavy
chain constant regions, and such sequences can be expressed in a cell that expresses an
immunoglobulin light chain. A typical bispecific antibody has two heavy chains each having
three heavy chain CDRs, followed by (N-terminal to C-terminal) a C 1 domain, a hinge, a
C 2 domain, and a C 3 domain, and an immunoglobulin light chain that either does not
confer epitope-binding specificity but that can associate with each heavy chain, or that can
associate with each heavy chain and that can bind one or more of the epitopes bound by the
heavy chain epitope-binding regions, or that can associate with each heavy chain and
enable binding or one or both of the heavy chains to one or both epitopes.
The term “cell” includes any cell that is suitable for expressing a recombinant
nucleic acid sequence. Cells include those of prokaryotes and eukaryotes (single-cell or
multiple-cell), bacterial cells (e.g., strains of E. coli, Bacillus spp., Streptomyces spp., etc.),
mycobacteria cells, fungal cells, yeast cells (e.g., S. cerevisiae, S. pombe, P. pastoris, P.
methanolica, etc.), plant cells, insect cells (e.g., SF-9, SF-21, baculovirus-infected insect
cells, Trichoplusia ni, etc.), non-human animal cells, human cells, or cell fusions such as, for
example, hybridomas or quadromas. In some embodiments, the cell is a human, monkey,
ape, hamster, rat, or mouse cell. In some embodiments, the cell is eukaryotic and is
selected from the following cells: CHO (e.g., CHO K1, DXB-11 CHO, Veggie-CHO), COS
(e.g., COS-7), retinal cell, Vero, CV1, kidney (e.g., HEK293, 293 EBNA, MSR 293, MDCK,
HaK, BHK), HeLa, HepG2, WI38, MRC 5, Colo205, HB 8065, HL-60, (e.g., BHK21), Jurkat,
Daudi, A431 (epidermal), CV-1, U937, 3T3, L cell, C127 cell, SP2/0, NS-0, MMT 060562,
Sertoli cell, BRL 3A cell, HT1080 cell, myeloma cell, tumor cell, and a cell line derived from
an aforementioned cell. In some embodiments, the cell comprises one or more viral genes,
e.g., a retinal cell that expresses a viral gene (e.g., a PER.C6™ cell).
The phrase “complementarity determining region,” or the term “CDR,” includes an
amino acid sequence encoded by a nucleic acid sequence of an organism’s immunoglobulin
genes that normally (i.e., in a wild type animal) appears between two framework regions in a
variable region of a light or a heavy chain of an immunoglobulin molecule (e.g., an antibody
or a T cell receptor). A CDR can be encoded by, for example, a germline sequence or a
rearranged or unrearranged sequence, and, for example, by a naive or a mature B cell or a
T cell. A CDR can be somatically mutated (e.g., vary from a sequence encoded in an
animal’s germline), humanized, and/or modified with amino acid substitutions, additions, or
deletions. In some circumstances (e.g., for a CDR3), CDRs can be encoded by two or more
sequences (e.g., germline sequences) that are not contiguous (e.g., in an unrearranged
nucleic acid sequence) but are contiguous in a B cell nucleic acid sequence, e.g., as the
result of splicing or connecting the sequences (e.g., V-D-J recombination to form a heavy
chain CDR3).
The term "conservative,” when used to describe a conservative amino acid
substitution, includes substitution of an amino acid residue by another amino acid residue
having a side chain R group with similar chemical properties (e.g., charge or hydrophobicity).
In general, a conservative amino acid substitution will not substantially change the functional
properties of interest of a protein, for example, the ability of a variable region to specifically
bind a target epitope with a desired affinity. Examples of groups of amino acids that have
side chains with similar chemical properties include aliphatic side chains such as glycine,
alanine, valine, leucine, and isoleucine; aliphatic-hydroxyl side chains such as serine and
threonine; amide-containing side chains such as asparagine and glutamine; aromatic side
chains such as phenylalanine, tyrosine, and tryptophan; basic side chains such as lysine,
arginine, and histidine; acidic side chains such as aspartic acid and glutamic acid; and,
sulfur-containing side chains such as cysteine and methionine. Conservative amino acids
substitution groups include, for example, valine/leucine/isoleucine, phenylalanine/tyrosine,
lysine/arginine, alanine/valine, glutamate/aspartate, and asparagine/glutamine. In some
embodiments, a conservative amino acid substitution can be substitution of any native
residue in a protein with alanine, as used in, for example, alanine scanning mutagenesis. In
some embodiments, a conservative substitution is made that has a positive value in the
PAM250 log-likelihood matrix disclosed in Gonnet et al. (1992) Exhaustive Matching of the
Entire Protein Sequence Database, Science 256:1443-45, hereby incorporated by reference.
In some embodiments, the substitution is a moderately conservative substitution wherein the
substitution has a nonnegative value in the PAM250 log-likelihood matrix.
In some embodiments, residue positions in an immunoglobulin light chain or
heavy chain differ by one or more conservative amino acid substitutions. In some
embodiments, residue positions in an immunoglobulin light chain or functional fragment
thereof (e.g., a fragment that allows expression and secretion from, e.g., a B cell) are not
identical to a light chain whose amino acid sequence is listed herein, but differs by one or
more conservative amino acid substitutions.
The phrase “epitope-binding protein” includes a protein having at least one CDR
and that is capable of selectively recognizing an epitope, e.g., is capable of binding an
epitope with a K that is at about one micromolar or lower (e.g., a K that is about 1 x 10 M,
-7 -9 -9 -10 -11 -12
1 x 10 M, 1 x 10 M, 1 x 10 M, 1 x 10 M, 1 x 10 M, or about 1 x 10 M). Therapeutic
epitope-binding proteins (e.g., therapeutic antibodies) frequently require a K that is in the
nanomolar or the picomolar range.
The phrase “functional fragment” includes fragments of epitope-binding proteins
that can be expressed, secreted, and specifically bind to an epitope with a K in the
micromolar, nanomolar, or picomolar range. Specific recognition includes having a K that is
at least in the micromolar range, the nanomolar range, or the picomolar range.
The term “germline” includes reference to an immunoglobulin nucleic acid
sequence in a non-somatically mutated cell, e.g., a non-somatically mutated B cell or pre-B
cell or hematopoietic cell.
The phrase “heavy chain,” or “immunoglobulin heavy chain” includes an
immunoglobulin heavy chain constant region sequence from any organism. Heavy chain
variable domains include three heavy chain CDRs and four FR regions, unless otherwise
specified. Fragments of heavy chains include CDRs, CDRs and FRs, and combinations
thereof. A typical heavy chain has, following the variable domain (from N-terminal to C-
terminal), a C 1 domain, a hinge, a C 2 domain, and a C 3 domain. A functional fragment
H H H
of a heavy chain includes a fragment that is capable of specifically recognizing an epitope
(e.g., recognizing the epitope with a K in the micromolar, nanomolar, or picomolar range),
that is capable of expressing and secreting from a cell, and that comprises at least one CDR.
The term “identity” when used in connection with sequence includes identity as
determined by a number of different algorithms known in the art that can be used to measure
nucleotide and/or amino acid sequence identity. In some embodiments described herein,
identities are determined using a ClustalW v. 1.83 (slow) alignment employing an open gap
penalty of 10.0, an extend gap penalty of 0.1, and using a Gonnet similarity matrix
(MACVECTOR™ 10.0.2, MacVector Inc., 2008). The length of the sequences compared
with respect to identity of sequences will depend upon the particular sequences, but in the
case of a light chain constant domain, the length should contain sequence of sufficient
length to fold into a light chain constant domain that is capable of self-association to form a
canonical light chain constant domain, e.g., capable of forming two beta sheets comprising
beta strands and capable of interacting with at least one C 1 domain of a human or a
mouse. In the case of a C 1 domain, the length of sequence should contain sequence of
sufficient length to fold into a C 1 domain that is capable of forming two beta sheets
comprising beta strands and capable of interacting with at least one light chain constant
domain of a mouse or a human.
The phrase “immunoglobulin molecule” includes two immunoglobulin heavy
chains and two immunoglobulin light chains. The heavy chains may be identical or different,
and the light chains may be identical or different.
The phrase “light chain” includes an immunoglobulin light chain sequence from
any organism, and unless otherwise specified includes human and light chains and a
VpreB, as well as surrogate light chains. Light chain variable (V ) domains typically include
three light chain CDRs and four framework (FR) regions, unless otherwise specified.
Generally, a full-length light chain includes, from amino terminus to carboxyl terminus, a V
domain that includes FR1-CDR1-FR2-CDR2-FR3-CDR3-FR4, and a light chain constant
domain. Light chains include those, e.g., that do not selectively bind either a first or a
second epitope selectively bound by the epitope-binding protein in which they appear. Light
chains also include those that bind and recognize, or assist the heavy chain with binding and
recognizing, one or more epitopes selectively bound by the epitope-binding protein in which
they appear. Common light chains are those derived from a rearranged human V 1-39J 5
sequence or a rearranged human V 3-20J 1 sequence, and include somatically mutated
(e.g., affinity matured) versions.
The phrase “micromolar range” is intended to mean 1-999 micromolar; the
phrase “nanomolar range” is intended to mean 1-999 nanomolar; the phrase “picomolar
range” is intended to mean 1-999 picomolar.
The phrase “somatically mutated” includes reference to a nucleic acid sequence
from a B cell that has undergone class-switching, wherein the nucleic acid sequence of an
immunoglobulin variable region (e.g., a heavy chain variable domain or including a heavy
chain CDR or FR sequence) in the class-switched B cell is not identical to the nucleic acid
sequence in the B cell prior to class-switching, such as, for example, a difference in a CDR
or framework nucleic acid sequence between a B cell that has not undergone class-
switching and a B cell that has undergone class-switching. “Somatically mutated” includes
reference to nucleic acid sequences from affinity-matured B cells that are not identical to
corresponding immunoglobulin variable region sequences in B cells that are not affinity-
matured (i.e., sequences in the genome of germline cells). The phrase “somatically
mutated” also includes reference to an immunoglobulin variable region nucleic acid
sequence from a B cell after exposure of the B cell to an epitope of interest, wherein the
nucleic acid sequence differs from the corresponding nucleic acid sequence prior to
exposure of the B cell to the epitope of interest. The phrase “somatically mutated” refers to
sequences from antibodies that have been generated in an animal, e.g., a mouse having
human immunoglobulin variable region nucleic acid sequences, in response to an
immunogen challenge, and that result from the selection processes inherently operative in
such an animal.
The term “unrearranged,” with reference to a nucleic acid sequence, includes
nucleic acid sequences that exist in the germline of an animal cell.
The phrase “variable domain” includes an amino acid sequence of an
immunoglobulin light or heavy chain (modified as desired) that comprises the following
amino acid regions, in sequence from N-terminal to C-terminal (unless otherwise indicated):
FR1, CDR1, FR2, CDR2, FR3, CDR3, FR4.
Universal Light Chain
Prior efforts to make useful multispecific epitope-binding proteins, e.g., bispecific
antibodies, have been hindered by variety of problems that frequently share a common
paradigm: in vitro selection or manipulation of sequences to rationally engineer, or to
engineer through trial-and-error, a suitable format for pairing a heterodimeric bispecific
human immunoglobulin. Unfortunately, most if not all of the in vitro engineering approaches
provide largely ad hoc fixes that are suitable, if at all, for individual molecules. On the other
hand, in vivo methods for employing complex organisms to select appropriate pairings that
are capable of leading to human therapeutics have not been realized.
Mice containing human immunoglobulin loci, variable and constant regions
randomly inserted into the mouse genome, are known in the art. Initial strains of such mice
contained a limited number of human immunoglobulin gene segments. Specifically, a
handful of strains containing human immunoglobulin light chain gene segments contained
either one, three or four human immunoglobulin V gene segments and five human
immunoglobulin JL gene segments (Taylor et al. 1992, Nucleic Acids Research 20(23): 6287-
6295; Fishwild et al. 1996, Nature Biotechnology 14: 845-851; Lonberg et al. 1994, Nature
368: 856-859; Green et al. 1994, Nature Genetics 7:13-21; Green and Jakobovits 1998, J.
Exp. Med. 188(3): 483-495; Green 1999, J. Immunol. Methods 231: 11-23). These mice that
contained only a few human immunoglobulin V gene segments as part of fully human
transgenes randomly inserted into the mouse genome demonstrated compromised B cell
numbers, impaired B cell development and other immune deficiencies. Expression of the
human immunoglobulin V genes, as detected by surface expression of human C on B
cells, was lower than the endogenous light chain as compared to wild type. Surprisingly,
the present invention provides mice whose B cell numbers and development is nearly wild-
type in respects when mice are engineered at the endogenous immunoglobulin light chain
loci to contain either one or two human immunoglobulin V gene segments (e.g., Examples
2 and 14, Tables 3, 25 and 26, and FIGs. 4, 10A-18). Further, in some embodiments, mice
provided by the present invention, are able to generate several high-affinity reverse chimeric
antibodies containing human V and V domains in response to antigen, wherein the V
H L L
domains each contain one of two possible human V gene segments and one of five
possible human J gene segments (e.g., see Examples 5 – 10, 12, and 14). Thus, in
contrast to preliminary strains of mice engineered with human immunoglobulin light chain
miniloci (i.e., a limited number of human immunoglobulin gene segments), presently
provided engineered mice that contain a limited number of human immunoglobulin V gene
segments (either one or two) and, in some embodiments, two or more (e.g., 2, 3, 4, or 5)
human immunoglobulin J gene segments, surprisingly exhibit normal B cell numbers,
normal immunoglobulin light chain expression, and normal B cell development. Further,
such provided mice also show no reduced or impaired ability to mount robust immune
responses to multiple antigens as a result of a limited immunoglobulin light chain repertoire.
Accordingly, mice are provided that comprise a humanized V locus comprising no more
than two unrearranged human immunoglobulin V gene segments and two or more (e.g., 2,
3, 4, or 5) human immunoglobulin J gene segments—or no more than two rearranged
human V J segments—and that exhibit wild-type B cell populations in number, and exhibit
wild-type B cell development.
Generally, native mouse sequences are frequently not a good source for human
therapeutic sequences. For at least that reason, generating mouse heavy chain
immunoglobulin variable regions that pair with a common human light chain is of limited
practical utility. More in vitro engineering efforts would be expended in a trial-and-error
process to try to humanize the mouse heavy chain variable sequences while hoping to retain
epitope specificity and affinity while maintaining the ability to couple with the common human
light chain, with uncertain outcome. At the end of such a process, the final product may
maintain some of the specificity and affinity, and associate with the common light chain, but
ultimately immunogenicity in a human would likely remain a profound risk.
Therefore, a suitable mouse for making human therapeutics would include a
suitably large repertoire of human heavy chain variable region gene segments in place of
endogenous mouse heavy chain variable region gene segments. The human heavy chain
variable region gene segments should be able to rearrange and recombine with an
endogenous mouse heavy chain constant domain to form a reverse chimeric heavy chain
(i.e., a heavy chain comprising a human variable domain and a mouse constant region).
The heavy chain should be capable of class switching and somatic hypermutation so that a
suitably large repertoire of heavy chain variable domains are available for the mouse to
select one that can associate with the limited repertoire of human light chain variable
regions.
A mouse that selects a common light chain for a plurality of heavy chains has a
practical utility. In various embodiments, antibodies that express in a mouse that can only
express a common light chain will have heavy chains that can associate and express with an
identical or substantially identical light chain. This is particularly useful in making bispecific
antibodies. For example, such a mouse can be immunized with a first immunogen to
generate a B cell that expresses an antibody that specifically binds a first epitope. The
mouse (or a mouse genetically the same) can be immunized with a second immunogen to
generate a B cell that expresses an antibody that specifically binds the second epitope.
Variable heavy chain regions can be cloned from the B cells and expressed with the same
heavy chain constant region, and the same variable light chain region (e.g., a common light
chain) in a cell to make a bispecific antibody, wherein the variable heavy chain component of
the bispecific antibody has been selected by a mouse to associate and express with the
variable light chain (or common light chain) component.
The inventors have engineered a mouse for generating immunoglobulin light
chains that will suitably pair with a rather diverse family of heavy chains, including heavy
chains whose variable regions depart from germline sequences, e.g., affinity matured or
somatically mutated variable regions. In various embodiments, the mouse is devised to pair
human light chain variable domains with human heavy chain variable domains that comprise
somatic mutations, thus enabling a route to high affinity binding proteins suitable for use as
human therapeutics.
The genetically engineered mouse, through the long and complex process of
antibody selection within an organism, makes biologically appropriate choices in pairing a
diverse collection of human heavy chain variable domains with a limited number of human
light chain options. In order to achieve this, the mouse is engineered to present a limited
number of human light chain variable domain options in conjunction with a wide diversity of
human heavy chain variable domain options. Upon challenge with an immunogen, the
mouse maximizes the number of solutions in its repertoire to develop an antibody to the
immunogen, limited largely or solely by the number or light chain options in its repertoire. In
various embodiments, this includes allowing the mouse to achieve suitable and compatible
somatic mutations of the light chain variable domain that will nonetheless be compatible with
a relatively large variety of human heavy chain variable domains, including in particular
somatically mutated human heavy chain variable domains.
To achieve a limited repertoire of light chain options, the mouse is engineered to
render nonfunctional or substantially nonfunctional its ability to make, or rearrange, a native
mouse light chain variable domain. This can be achieved, e.g., by deleting the mouse’s light
chain variable region gene segments. The endogenous mouse locus can then be modified
by an exogenous suitable human light chain variable region gene segment of choice,
operably linked to the endogenous mouse light chain constant domain, in a manner such
that the exogenous human variable region gene segments can combine with the
endogenous mouse light chain constant region gene and form a rearranged reverse chimeric
light chain gene (human variable, mouse constant). In various embodiments, the light chain
variable region is capable of being somatically mutated. In various embodiments, to
maximize ability of the light chain variable region to acquire somatic mutations, the
appropriate enhancer(s) is retained in the mouse. For example, in modifying a mouse light
chain locus to replace endogenous mouse light chain gene segments with human light
chain gene segments, the mouse intronic enhancer and mouse 3’ enhancer are
functionally maintained, or undisrupted.
A genetically engineered mouse is provided that expresses a limited repertoire of
reverse chimeric (human variable, mouse constant) light chains associated with a diversity of
reverse chimeric (human variable, mouse constant) heavy chains. In various embodiments,
the endogenous mouse light chain gene segments are deleted and replaced with a single
(or two) rearranged human light chain region, operably linked to the endogenous mouse C
gene. In embodiments for maximizing somatic hypermutation of the rearranged human light
chain region, the mouse intronic enhancer and the mouse 3’ enhancer are maintained.
In various embodiments, the mouse also comprises a nonfunctional light chain locus, or a
deletion thereof or a deletion that renders the locus unable to make a light chain.
A genetically engineered mouse is provided that, in various embodiments,
comprises a light chain variable region locus lacking endogenous mouse light chain V and
J gene segments and comprising a rearranged human light chain variable region, in one
embodiment a rearranged human V /J sequence, operably linked to a mouse constant
region, wherein the locus is capable of undergoing somatic hypermutation, and wherein the
locus expresses a light chain comprising the human V /J sequence linked to a mouse
constant region. Thus, in various embodiments, the locus comprises a mouse 3’
enhancer, which is correlated with a normal, or wild type, level of somatic hypermutation.
The genetically engineered mouse in various embodiments when immunized with
an antigen of interest generates B cells that exhibit a diversity of rearrangements of human
immunoglobulin heavy chain variable regions that express and function with one or with two
rearranged light chains, including embodiments where the one or two light chains comprise
human light chain variable regions that comprise, e.g., 1 to 5 somatic mutations. In various
embodiments, the human light chains so expressed are capable of associating and
expressing with any human immunoglobulin heavy chain variable region expressed in the
mouse.
In addition to genetically engineered mice comprising restricted immunoglobulin
light chain repertoire (e.g., a single human V gene segment or no more than two human V
gene segments and, one human J gene segment or, optionally, two or more human J gene
segments) as described herein, also provided herein are other genetically modified non-
human animals that comprise a single human V gene segment or no more than two human
V gene segments. In some embodiments, such non-human animals comprise a single
rearranged human V region composed of a rearranged human V J sequence. In some
L L L
embodiments, such non-human animals comprise no more than two human V gene
segments and two or more (e.g., 2, 3, 4, or 5 human J gene segments. In various
embodiments, human gene segments are operably linked to a non-human light chain
constant region, e.g., a mouse a rat light chain constant region.
Such non-human animals may be selected from a group consisting of a mouse,
rat, rabbit, pig, bovine (e.g., cow, bull, buffalo), deer, sheep, goat, chicken, cat, dog, ferret,
primate (e.g., marmoset, rhesus monkey). For the non-human animals where suitable
genetically modifiable ES cells are not readily available, other methods are employed to
make a non-human animal comprising genetic modifications as described herein. Such
methods include, e.g., modifying a non-ES cell genome (e.g., a fibroblast or an induced
pluripotent cell) and employing nuclear transfer to transfer the modified genome to a suitable
cell, e.g., an oocyte, and gestating the modified cell (e.g., the modified oocyte) in a non-
human animal under suitable conditions to form an embryo.
In some embodiments, a non-human animal of the present invention is a
mammal. In some embodiments, a non-human animal of the present invention is a small
mammal, e.g., of the superfamily Dipodoidea or Muroidea. In some embodiments, a
genetically modified animal of the present invention is a rodent. In some embodiments, a
rodent of the present invention is selected from a mouse, a rat, and a hamster. In some
embodiments, a rodent of the present invention is selected from the superfamily Muroidea.
In some embodiments, a genetically modified animal of the present invention is from a family
selected from Calomyscidae (e.g., mouse-like hamsters), Cricetidae (e.g., hamster, New
World rats and mice, voles), Muridae (true mice and rats, gerbils, spiny mice, crested rats),
Nesomyidae (climbing mice, rock mice, with-tailed rats, Malagasy rats and mice),
Platacanthomyidae (e.g., spiny dormice), and Spalacidae (e.g., mole rates, bamboo rats,
and zokors). In some certain embodiments, a genetically modified rodent of the present
invention is selected from a true mouse or rat (family Muridae), a gerbil, a spiny mouse, and
a crested rat. In some certain embodiments, a genetically modified mouse of the present
invention is from a member of the family Muridae. In some embodiment, an non-human
animal of the present invention is a rodent. In some certain embodiments, a rodent of the
present invention is selected from a mouse and a rat. In some embodiments, a non-human
animal of the present invention is a mouse.
In some embodiments, a non-human animal of the present invention is a rodent
that is a mouse of a C57BL strain selected from C57BL/A, C57BL/An, C57BL/GrFa,
C57BL/KaLwN, C57BL/6, C57BL/6J, C57BL/6ByJ, C57BL/6NJ, C57BL/10, C57BL/10ScSn,
C57BL/10Cr, and C57BL/Ola. In some certain embodiments, a mouse of the present
invention is a 129 strain selected from the group consisting of a strain that is 129P1, 129P2,
129P3,129X1, 129S1 (e.g., 129S1/SV, 129S1/SvIm), 129S2, 129S4, 129S5, 129S9/SvEvH,
129S6 (129/SvEvTac), 129S7, 129S8, 129T1, 129T2 (see, e.g., Festing et al., 1999,
Mammalian Genome 10:836; Auerbach et al., 2000, Biotechniques 29(5):1024-1028, 1030,
1032). In some certain embodiments, a genetically modified mouse of the present invention
is a mix of an aforementioned 129 strain and an aforementioned C57BL/6 strain. In some
certain embodiments, a mouse of the present invention is a mix of aforementioned 129
strains, or a mix of aforementioned BL/6 strains. In some certain embodiments, a 129 strain
of the mix as described herein is a 129S6 (129/SvEvTac) strain. In some embodiment, a
mouse of the present invention is a BALB strain, e.g., BALB/c strain. In some embodiments,
a mouse of the present invention is a mix of a BALB strain and another aforementioned
strain.
In some embodiments, a non-human animal of the present invention is a rat. In
some certain embodiments, a rat of the present invention is selected from a Wistar rat, an
LEA strain, a Sprague Dawley strain, a Fischer strain, F344, F6, and Dark Agouti. In some
certain embodiments, a rat strain as described herein is a mix of two or more strains
selected from the group consisting of Wistar, LEA, Sprague Dawley, Fischer, F344, F6, and
Dark Agouti.
Epitope-binding Proteins Binding More Than One Epitope
Compositions and methods described herein can be used to make binding
proteins that bind more than one epitope with high affinity, e.g., bispecific antibodies.
Advantages of the invention include the ability to select suitably high binding (e.g., affinity
matured) heavy chain immunoglobulin chains each of which will associate with a single light
chain.
Several techniques for making bispecific antibody fragments from recombinant
cell culture have been reported. However, synthesis and expression of bispecific binding
proteins has been problematic, in part due to issues associated with identifying a suitable
light chain that can associate and express with two different heavy chains, and in part due to
isolation issues. In various embodiments, compositions and methods described herein
provide the advantage of full length bispecific antibodies that do not require special
modification(s) to maintain traditional immunoglobulin structure by increasing
stability/interaction of the components (). In various embodiments, such
modification(s) has proven cumbersome and served as an obstacle to development of
bispecific antibody technology and their potential use in treating for human disease. Thus, in
various embodiments, through providing a natural immunoglobulin structure (i.e., full length)
having the added property of multiple specificities, full length bispecific antibodies maintain
their critical effector functions that previous bispecific fragments lack, and further provide
therapeutics that demonstrate the important pharmacokinetic parameter of a longer half-life.
Methods and compositions described herein allow for a genetically modified
mouse to select, through otherwise natural processes, a suitable light chain that can
associate and express with more than one heavy chain, including heavy chains that are
somatically mutated (e.g., affinity matured). Human V and V sequences from suitable B
cells of immunized mice as described herein that express affinity matured antibodies having
reverse chimeric heavy chains (i.e., human variable and mouse constant) can be identified
and cloned in frame in an expression vector with a suitable human constant region gene
sequence (e.g., a human IgG1). Two such constructs can be prepared, wherein each
construct encodes a human heavy chain variable domain that binds a different epitope. One
of the human V s (e.g., human V 1-39J 5 or human V 3-20J 1), in germline sequence or
from a B cell wherein the sequence has been somatically mutated, can be fused in frame to
a suitable human constant region gene (e.g., a human constant gene). These three fully
human heavy and light constructs can be placed in a suitable cell for expression. The cell
will express two major species: a homodimeric heavy chain with the identical light chain,
and a heterodimeric heavy chain with the identical light chain. To allow for a facile
separation of these major species, one of the heavy chains is modified to omit a Protein A-
binding determinant, resulting in a differential affinity of a homodimeric binding protein from a
heterodimeric binding protein. Compositions and methods that address this issue are
described in USSN 12/832,838, filed 25 June 2010, entitled “Readily Isolated Bispecific
Antibodies with Native Immunoglobulin Format,” published as US 2010/0331527A1, hereby
incorporated by reference.
In one aspect, an epitope-binding protein as described herein is provided,
wherein human V and V sequences are derived from mice described herein that have
been immunized with an antigen comprising an epitope of interest.
In one embodiment, an epitope-binding protein is provided that comprises a first
and a second polypeptide, the first polypeptide comprising, from N-terminal to C-terminal, a
first epitope-binding region that selectively binds a first epitope, followed by a constant
region that comprises a first C 3 region of a human IgG selected from IgG1, IgG2, IgG4, and
a combination thereof; and, a second polypeptide comprising, from N-terminal to C-terminal,
a second epitope-binding region that selectively binds a second epitope, followed by a
constant region that comprises a second C 3 region of a human IgG selected from IgG1,
IgG2, IgG4, and a combination thereof, wherein the second C 3 region comprises a
modification that reduces or eliminates binding of the second C 3 domain to protein A.
In one embodiment, the second C 3 region comprises an H95R modification (by
IMGT exon numbering; H435R by EU numbering). In another embodiment, the second CH3
region further comprises a Y96F modification (IMGT; Y436F by EU).
In one embodiment, the second C 3 region is from a modified human IgG1, and
further comprises a modification selected from the group consisting of D16E, L18M, N44S,
K52N, V57M, and V82I (IMGT; D356E, L358M, N384S, K392N, V397M, and V422I by EU).
In one embodiment, the second C 3 region is from a modified human IgG2, and
further comprises a modification selected from the group consisting of N44S, K52N, and
V82I (IMGT; N384S, K392N, and V422I by EU).
In one embodiment, the second C 3 region is from a modified human IgG4, and
further comprises a modification selected from the group consisting of Q15R, N44S, K52N,
V57M, R69K, E79Q, and V82I (IMGT; Q355R, N384S, K392N, V397M, R409K, E419Q, and
V422I by EU).
One method for making an epitope-binding protein that binds more than one
epitope is to immunize a first mouse in accordance with the invention with an antigen that
comprises a first epitope of interest, wherein the mouse comprises an endogenous
immunoglobulin light chain variable region locus that does not contain an endogenous
mouse V that is capable of rearranging and forming a light chain, wherein at the
endogenous mouse immunoglobulin light chain variable region locus is a single rearranged
human V region operably linked to the mouse endogenous light chain constant region gene,
and the rearranged human V region is selected from a human V 1-39J 5 and a human
V 3-20J 1, and the endogenous mouse V gene segments have been replaced in whole or
in part with human V gene segments, such that immunoglobulin heavy chains made by the
mouse are solely or substantially heavy chains that comprise human variable domains and
mouse constant domains. When immunized, such a mouse will make a reverse chimeric
antibody, comprising only one of two human light chain variable domains (e.g., one of
human V 1-39J 5 or human V 3-20J 1). Once a B cell is identified that encodes a VH that
binds the epitope of interest, the nucleotide sequence of the V (and, optionally, the V ) can
be retrieved (e.g., by PCR) and cloned into an expression construct in frame with a suitable
human immunoglobulin constant domain. This process can be repeated to identify a second
V domain that binds a second epitope, and a second V gene sequence can be retrieved
and cloned into an expression vector in frame to a second suitable immunoglobulin constant
domain. The first and the second immunoglobulin constant domains can the same or
different isotype, and one of the immunoglobulin constant domains (but not the other) can be
modified as described herein or in US 2010/0331527A1, and epitope-binding protein can be
expressed in a suitable cell and isolated based on its differential affinity for Protein A as
compared to a homodimeric epitope-binding protein, e.g., as described in US
2010/0331527A1.
In one embodiment, a method for making a bispecific epitope-binding protein is
provided, comprising identifying a first affinity-matured (e.g., comprising one or more somatic
hypermutations) human V nucleotide sequence (V 1) from a mouse as described herein,
identifying a second affinity-matured (e.g., comprising one or more somatic hypermutations)
human V nucleotide sequence (V 2) from a mouse as described herein, cloning V 1 in
H H H
frame with a human heavy chain lacking a Protein A-determinant modification as described
in US 2010/0331527A1 for form heavy chain 1 (HC1), cloning V 2 in frame with a human
heavy chain comprising a Protein A-determinant as described in US 2010/0331527A1 to
form heavy chain 2 (HC2), introducing an expression vector comprising HC1 and the same
or a different expression vector comprising HC2 into a cell, wherein the cell also expresses a
human immunoglobulin light chain that comprises a human V 1-39/human J 5 or a human
V 3-20/human J 1 fused to a human light chain constant domain, allowing the cell to
express a bispecific epitope-binding protein comprising a V domain encoded by V 1 and a
V domain encoded by V 2, and isolating the bispecific epitope-binding protein based on its
differential ability to bind Protein A as compared with a monospecific homodimeric epitope-
binding protein. In a specific embodiment, HC1 is an IgG1, and HC2 is an IgG1 that
comprises the modification H95R (IMGT; H435R by EU) and further comprises the
modification Y96F (IMGT; Y436F by EU). In one embodiment, the VH domain encoded by
V 1, the V domain encoded by V 2, or both, are somatically mutated.
H H H
Human V Genes That Express with a Common Human V
A variety of human variable regions from affinity-matured antibodies raised
against four different antigens were expressed with either their cognate light chain, or at
least one of a human light chain selected from human V 1-39/J 5, human V 3-20/J 1, or
human VpreB/J 5 (see Example 1). For antibodies to each of the antigens, somatically
mutated high affinity heavy chains from different gene families paired successfully with
rearranged human germline V 1-39J 5 and V 3-20J 1 regions and were secreted from
cells expressing the heavy and light chains. For V 1-39J 5 and V 3-20J 1, V domains
derived from the following human V gene families expressed favorably: 1-2, 1-8, 1-24, 2-5,
3-7, 3-9, 3-11, 3-13, 3-15, 3-20, 3-23, 3-30, 3-33, 3-48, 4-31, 4-39, 4-59, 5-51, and 6-1.
Thus, a mouse that is engineered to express a limited repertoire of human V domains from
one or both of V 1-39J 5 and V 3-20J 1 will generate a diverse population of somatically
mutated human V domains from a V locus modified to replace mouse V gene segments
H H H
with human V gene segments.
Mice genetically engineered to express reverse chimeric (human variable, mouse
constant) immunoglobulin heavy chains associated with a single rearranged light chain (e.g.,
a V 1-39/J or a V 3-20/J), when immunized with an antigen of interest, generated B cells
that comprised a diversity of human V rearrangements and expressed a diversity of high-
affinity antigen-specific antibodies with diverse properties with respect to their ability to block
binding of the antigen to its ligand, and with respect to their ability to bind variants of the
antigen (see Examples 5 through 10).
Thus, the mice and methods described herein are useful in making and selecting
human immunoglobulin heavy chain variable domains, including somatically mutated human
heavy chain variable domains, that result from a diversity of rearrangements, that exhibit a
wide variety of affinities (including exhibiting a K of about a nanomolar or less), a wide
variety of specificities (including binding to different epitopes of the same antigen), and that
associate and express with the same or substantially the same human immunoglobulin light
chain variable region.
Fully Human Bispecific Antibodies Having a Common Light Chain
As a first step in various embodiments, the first and second nucleic acid
sequences that each encode human heavy chain variable domains (and any additional
nucleic acid sequences forming the bispecific antibody) are selected from parent monoclonal
antibodies having desired characteristics such as, for example, capable of binding different
epitopes (see FIGs. 7A and 7B), having different affinities, etc. Normally, the nucleic acid
sequences encoding the human heavy chain variable domains are isolated from immunized
mice, as described herein, to allow for fusing with human heavy chain constant regions to be
suitable for human administration. Further modifications to the sequence(s) can be made by
introducing mutations that add additional functionality to the bispecific antibody can be
achieved, which include, for example, increasing serum half-life (e.g., see U.S. 7,217,797)
and/or increasing antibody-dependent cell-mediated cytotoxicity (e.g., see U.S. 6,737,056).
Introducing mutations into the constant regions of antibodies is known in the art.
Additionally, part of the bispecific antibody can be made recombinantly in cell culture and
other part(s) of the molecule can be made by those techniques mentioned above.
Several techniques for the producing antibodies have been described. For
example, in various embodiments chimeric antibodies are produced in mice as described
herein. Antibodies can be isolated directly from B cells of an immunized mouse (e.g., see
U.S. 2007/0280945A1) and/or the B cells of the immunized mouse can be used to make
hybridomas (Kohler and Milstein, 1975, Nature 256:495-497). DNA encoding the antibodies
(human heavy and/or light chains) from mice as described herein is readily isolated and
sequenced using conventional techniques. Hybridoma and/or B cells of derived from mice
as described herein serve as a preferred source of such DNA. Once isolated, the DNA may
be placed into expression vectors, which are then transfected into host cells that do not
otherwise produce immunoglobulin protein, to obtain the synthesis of monoclonal antibodies
in the recombinant host cells. The DNA also may be modified, for example, by substituting
the coding sequence for human heavy and light chain constant domains in place of the
murine sequences.
In various embodiments, following isolation of the DNA and selection of the first
and second nucleic acid sequences that encode the first and second human heavy chain
variable domains having the desired specificities/affinities, and a third nucleic acid sequence
that encodes a human light chain domain (a germline rearranged sequence or a light chain
sequence isolated from a mouse as described herein), the three nucleic acids sequences
encoding the molecules are expressed to form the bispecific antibody using recombinant
techniques which are widely available in the art. Often, the expression system of choice will
involve a mammalian cell expression vector and host so that the bispecific antibody is
appropriately glycosylated (e.g., in the case of bispecific antibodies comprising antibody
domains which are glycosylated). However, the molecules can also be produced in the
prokaryotic expression systems. Normally, the host cell will be transformed with DNA
encoding both the first human heavy chain variable domain, the second human heavy chain
variable domain, the human light chain domain on a single vector or independent vectors.
However, it is possible to express the first human heavy chain variable domain, second
human heavy chain variable domain, and human light chain domain (the bispecific antibody
components) in independent expression systems and couple the expressed polypeptides in
vitro. In various embodiments, the human light chain domain comprises a germline
sequence. In various embodiments, the human light chain domain comprises no more than
one, no more than two, no more than three, no more than four, or no more than five somatic
hypermutations with the light chain variable sequence of the light chain domain.
In various embodiments, the nucleic acid(s) (e.g., cDNA or genomic DNA)
encoding the two heavy chains and single human light chain is inserted into a replicable
vector for further cloning (amplification of the DNA) and/or for expression. Many vectors are
available, and generally include, but are not limited to, one or more of the following: a signal
sequence, an origin of replication, one or more marker genes, an enhancer element, a
promoter, and a transcription termination sequence. Each component may be selected
individually or based on a host cell choice or other criteria determined experimentally.
Several examples of each component are known in the art.
Expression and cloning vectors usually contain a promoter that is recognized by
the host organism and is operably linked to the nucleic acid sequences that encode each or
all the components of the bispecific antibody. A large number of promoters recognized by a
variety of potential host cells are well known. These promoters are operably linked to
bispecific antibody-encoding DNA by removing the promoter from the source DNA by
restriction enzyme digestion and inserting the isolated promoter sequence into the vector.
Expression vectors used in eukaryotic host cells (yeast, fungi, insect, plant,
animal, human, or nucleated cells from other multicellular organisms) may also contain
sequences necessary for the termination of transcription and for stabilizing the mRNA. Such
sequences are commonly available from the 5' and, occasionally 3', untranslated regions of
eukaryotic or viral DNAs or cDNAs. These regions contain nucleotide segments transcribed
as polyadenylated fragments in the untranslated portion of the mRNA encoding the bispecific
antibody components. Suitable expression vectors for various embodiments include those
that provide for the transient expression in mammalian cells of DNA encoding the bispecific
antibody. In general, transient expression involves the use of an expression vector that is
able to replicate efficiently in a host cell, such that the host cell accumulates many copies of
the expression vector and, in turn, synthesizes high levels of a desired polypeptide encoded
by the expression vector. Transient expression systems, comprising a suitable expression
vector and a host cell, allow for the convenient positive identification of polypeptides
encoded by cloned DNAs, as well as for the rapid screening of bispecific antibodies having
desired binding specificities/affinities or the desired gel migration characteristics relative to
the parental antibodies having homodimers of the first or second human heavy chain
variable domains.
In various embodiments, once the DNA encoding the components of the
bispecific antibody are assembled into the desired vector(s) as described above, they are
introduced into a suitable host cell for expression and recovery. Transfecting host cells can
be accomplished using standard techniques known in the art appropriate to the host cell
selected (e.g., electroporation, nuclear microinjection, bacterial protoplast fusion with intact
cells, or polycations, e.g., polybrene, polyornithine, etc.).
A host cell is chosen, in various embodiments, that best suits the expression
vector containing the components and allows for the most efficient and favorable production
of the bispecific antibody species. Exemplary host cells for expression include those of
prokaryotes and eukaryotes (single-cell or multiple-cell), bacterial cells (e.g., strains of E.
coli, Bacillus spp., Streptomyces spp., etc.), mycobacteria cells, fungal cells, yeast cells
(e.g., S. cerevisiae, S. pombe, P. pastoris, P. methanolica, etc.), plant cells, insect cells
(e.g., SF-9, SF-21, baculovirus-infected insect cells, Trichoplusia ni, etc.), non-human animal
cells, human cells, or cell fusions such as, for example, hybridomas or quadromas. In
various embodiments, the cell is a human, monkey, ape, hamster, rat, or mouse cell. In
various embodiments, the cell is eukaryotic cell selected from CHO (e.g., CHO K1, DXB-11
CHO, Veggie-CHO), COS (e.g., COS-7), retinal cell, Vero, CV1, kidney (e.g., HEK293, 293
EBNA, MSR 293, MDCK, HaK, BHK), HeLa, HepG2, WI38, MRC 5, Colo205, HB 8065, HL-
60, (e.g., BHK21), Jurkat, Daudi, A431 (epidermal), CV-1, U937, 3T3, L cell, C127 cell,
SP2/0, NS-0, MMT 060562, Sertoli cell, BRL 3A cell, HT1080 cell, myeloma cell, tumor cell,
and a cell line derived from an aforementioned cell. In various embodiments, the cell
comprises one or more viral genes, e.g. a retinal cell that expresses a viral gene (e.g., a
PER.C6™ cell).
Mammalian host cells used to produce the bispecific antibody may be cultured in
a variety of media. Commercially available media such as Ham's F10 (Sigma), Minimal
Essential Medium ((MEM), Sigma), RPMI-1640 (Sigma), and Dulbeccols Modified Eagle's
Medium ((DMEM), Sigma) are suitable for culturing the host cells. Media may be
supplemented as necessary with hormones and/or other growth factors (such as insulin,
transferrin, or epidermal growth factor), salts (such as sodium chloride, calcium, magnesium,
and phosphate), buffers (such as HEPES), nucleosides (such as adenosine and thymidine),
antibiotics (such as GENTAMYCIN ), trace elements (defined as inorganic compounds
usually present at final concentrations in the micromolar range), and glucose or an
equivalent energy source. Any other supplements may also be included at appropriate
concentrations as known to those skilled in the art. The culture conditions, such as
temperature, pH, and the like, are, in various embodiments, those previously used with the
host cell selected for expression, and will be apparent to those skilled in the art.
The bispecific antibody is in various embodiments recovered from the culture
medium as a secreted polypeptide, although it also may be recovered from host cell lysate
when directly produced without a secretory signal. If the bispecific antibody is membrane-
bound, it can be released from the membrane using a suitable detergent solution (e.g.,
Triton-X 100). Preferably, the bispecific antibodies described herein involves the use of a
first immunoglobulin C 3 domain and a second immunoglobulin C 3 domain, wherein the
first and second immunoglobulin C 3 domains differ from one another by at least one amino
acid, and wherein at least one amino acid difference reduces binding of the bispecific
antibody to Protein A as compared to a bi-specific antibody lacking the amino acid difference
(see U.S. 2010/0331527A1; herein incorporated by reference). In one embodiment, the first
immunoglobulin C 3 domain binds Protein A and the second immunoglobulin C 3 domain
contains a mutation that reduces or abolishes Protein A binding such as an H95R
modification (by IMGT exon numbering; H435R by EU numbering). The second C 3 may
further comprise a Y96F modification (by IMGT; Y436F by EU). Further modifications that
may be found within the second C 3 include: D16E, L18M, N44S, K52N, V57M, and V82I
(by IMGT; D356E, L358M, N384S, K392N, V397M, and V422I by EU) in the case of IgG1
antibodies; N44S, K52N, and V82I (IMGT; N384S, K392N, and V422I by EU) in the case of
IgG2 antibodies; and Q15R, N44S, K52N, V57M, R69K, E79Q, and V82I (by IMGT; Q355R,
N384S, K392N, V397M, R409K, E419Q, and V422I by EU) in the case of IgG4 antibodies.
Variations on the bi-specific antibody format described above are contemplated within the
scope of the present invention.
Because of the dual nature of bispecific antibodies (i.e., may be specific for
different epitopes of one polypeptide or may contain antigen-binding domains specific for
more than one target polypeptide, see ; see also, e.g., Tutt et al., 1991, J. Immunol.
147:60-69; Kufer et al., 2004, Trends Biotechnol. 22:238-244), they offer many useful
advantages for therapeutic application. For example, the bispecific antibodies can be used
for redirected cytotoxicity (e.g., to kill tumor cells), as a vaccine adjuvant, for delivering
thrombolytic agents to clots, for converting enzyme activated prodrugs at a target site (e.g., a
tumor), for treating infectious diseases, targeting immune complexes to cell surface
receptors, or for delivering immunotoxins to tumor cells.
The bispecific antibodies described herein can also be used in several
therapeutic and non-therapeutic and/or diagnostic assay methods, such as, enzyme
immunoassays, two-site immunoassays, in vitro or in vivo immunodiagnosis of various
diseases (e.g., cancer), competitive binding assays, direct and indirect sandwich assays,
and immunoprecipitation assays. Other uses for the bispecific antibodies will be apparent to
those skilled in the art.
The following examples are provided so as to describe to those of ordinary skill in
the art how to make and use methods and compositions of the invention, and are not
intended to limit the scope of what the inventors regard as their invention. Efforts have been
made to ensure accuracy with respect to numbers used (e.g., amounts, temperature, etc.)
but some experimental errors and deviations should be accounted for. Unless indicated
otherwise, parts are parts by weight, molecular weight is average molecular weight,
temperature is indicated in Celsius, and pressure is at or near atmospheric.
EXAMPLES
The following examples are provided so as to describe to those of ordinary skill in
the art how to make and use methods and compositions of the invention, and are not
intended to limit the scope of what the inventors regard as their invention. Efforts have been
made to ensure accuracy with respect to numbers used (e.g., amounts, temperature, etc.)
but some experimental errors and deviations should be accounted for. Unless indicated
otherwise, temperature is indicated in Celsius, pressure is at or near atmospheric, parts are
by parts by weight, and molecular weight is average molecular weight.
Example 1. Identification of Human V Regions That Associate with Selected Human
V Regions
An in vitro expression system was constructed to determine if a single rearranged
human germline light chain could be co-expressed with human heavy chains from antigen
specific human antibodies.
Methods for generating human antibodies in genetically modified mice are known
(see e.g., US 6,596,541, Regeneron Pharmaceuticals, VELOCIMMUNE®). The
VELOCIMMUNE® technology involves generation of a genetically modified mouse having a
genome comprising human heavy and light chain variable regions operably linked to
endogenous mouse constant region loci such that the mouse produces an antibody
comprising a human variable region and a mouse constant region in response to antigenic
stimulation. The DNA encoding the variable regions of the heavy and light chains of the
antibodies produced from a VELOCIMMUNE® mouse are fully human. Initially, high affinity
chimeric antibodies are isolated having a human variable region and a mouse constant
region. As described below, the antibodies are characterized and selected for desirable
characteristics, including affinity, selectivity, epitope, etc. The mouse constant regions are
replaced with a desired human constant region to generate a fully human antibody
containing a non-IgM isotype, for example, wild type or modified IgG1, IgG2, IgG3 or IgG4.
While the constant region selected may vary according to specific use, high affinity antigen-
binding and target specificity characteristics reside in the variable region.
A VELOCIMMUNE® mouse was immunized with a growth factor that promotes
angiogenesis (Antigen C) and antigen-specific human antibodies were isolated and
sequenced for V gene usage using standard techniques recognized in the art. Selected
antibodies were cloned onto human heavy and light chain constant regions and 69 heavy
chains were selected for pairing with one of three human light chains: (1) the cognate light
chain linked to a human constant region, (2) a rearranged human germline V 1-39J 5
linked to a human constant region, or (3) a rearranged human germline V 3-20J 1 linked
to a human constant region. Each heavy chain and light chain pair was co-transfected in
CHO-K1 cells using standard techniques. Presence of antibody in the supernatant was
detected by anti-human IgG in an ELISA assay. Antibody titer (ng/ml) was determined for
each heavy chain/light chain pair and titers with the different rearranged germline light
chains were compared to the titers obtained with the parental antibody molecule (i.e., heavy
chain paired with cognate light chain) and percent of native titer was calculated (Table 1).
V : Heavy chain variable gene. ND: no expression detected under current experimental
conditions.
TABLE 1
Antibody Titer (ng/mL) Percent of Native Titer
Cognate LC V 1-39J 5 V 3-20J 1 V 1-39J 5 V 3-20J 1
3-15 63 23 11 36.2 17.5
1-2 103 53 ND 51.1 -
3-23 83 60 23 72.0 27.5
3-33 15 77 ND 499.4 -
4-31 22 69 17 309.4 76.7
3-7 53 35 28 65.2 53.1
- 22 32 19 148.8 89.3
1-24 3 13 ND 455.2 -
3-33 1 47 ND 5266.7 -
3-33 58 37 ND 63.1 -
- 110 67 18 60.6 16.5
3-23 127 123 21 96.5 16.3
3-33 28 16 2 57.7 7.1
3-23 32 50 38 157.1 119.4
- 18 45 18 254.3 101.7
3-9 1 30 23 2508.3 1900.0
3-11 12 26 6 225.9 48.3
1-8 16 ND 13 - 81.8
3-33 54 81 10 150.7 19.1
- 34 9 ND 25.9 -
3-20 7 14 54 203.0 809.0
3-33 19 38 ND 200.5 -
3-11 48 ND 203 - 423.6
- 11 23 8 212.7 74.5
3-33 168 138 182 82.0 108.2
3-20 117 67 100 57.5 86.1
3-23 86 61 132 70.7 154.1
3-33 20 12 33 60.9 165.3
4-31 69 92 52 133.8 75.0
3-23 87 78 62 89.5 71.2
1-2 31 82 51 263.0 164.6
3-23 53 93 151 175.4 285.4
- 11 8 17 75.7 151.4
3-33 114 36 27 31.6 23.4
3-15 73 39 44 53.7 59.6
3-33 1 34 16 5600.0 2683.3
3-9 58 112 57 192.9 97.6
3-33 67 20 105 30.1 157.0
3-33 34 21 24 62.7 70.4
3-20 10 49 91 478.4 888.2
3-33 66 32 25 48.6 38.2
3-23 17 59 56 342.7 329.8
- 58 108 19 184.4 32.9
- 68 54 20 79.4 29.9
3-33 42 35 32 83.3 75.4
- 29 19 13 67.1 43.9
3-9 24 34 29 137.3 118.4
3-30/33 17 33 7 195.2 43.1
3-7 25 70 74 284.6 301.6
3-33 87 127 ND 145.1 -
6-1 28 56 ND 201.8 -
3-33 56 39 20 69.9 36.1
3-33 10 53 1 520.6 6.9
3-33 20 67 10 337.2 52.3
3-33 11 36 18 316.8 158.4
3-23 12 42 32 356.8 272.9
3-33 66 95 15 143.6 22.5
3-15 55 68 ND 123.1 -
- 32 68 3 210.9 10.6
1-8 28 48 ND 170.9 -
3-33 124 192 21 154.3 17.0
3-33 0 113 ND 56550.0 -
3-33 10 157 1 1505.8 12.5
3-33 6 86 15 1385.5 243.5
3-23 70 115 22 163.5 31.0
3-7 71 117 21 164.6 29.6
3-33 82 100 47 122.7 57.1
3-7 124 161 41 130.0 33.5
In a similar experiment, VELOCIMMUNE® mice were immunized with several
different antigens and selected heavy chains of antigen specific human antibodies were
tested for their ability to pair with different rearranged human germline light chains (as
described above). The antigens used in this experiment included an enzyme involved in
cholesterol homeostasis (Antigen A), a serum hormone involved in regulating glucose
homeostasis (Antigen B), a growth factor that promotes angiogenesis (Antigen C) and a cell-
surface receptor (Antigen D). Antigen specific antibodies were isolated from mice of each
immunization group and the heavy chain and light chain variable regions were cloned and
sequenced. From the sequence of the heavy and light chains, V gene usage was
determined and selected heavy chains were paired with either their cognate light chain or a
rearranged human germline V 1-39J 5 region. Each heavy/light chain pair was co-
transfected in CHO-K1 cells and the presence of antibody in the supernatant was detected
by anti-human IgG in an ELISA assay. Antibody titer (µg/ml) was determined for each heavy
chain/light chain pairing and titers with the different rearranged human germline light chains
were compared to the titers obtained with the parental antibody molecule (i.e., heavy chain
paired with cognate light chain) and percent of native titer was calculated (Table 2). V :
Heavy chain variable gene. V : light chain variable gene. ND: no expression detected
under current experimental conditions.
TABLE 2
Titer (µg/ml)
Percent of
Antigen Antibody V
H V V +
Native Titer
V Alone V + V
V 1-39J 5
320 1-18 2-30 0.3 3.1 2.0 66
321 2-5 2-28 0.4 0.4 1.9 448
334 2-5 2-28 0.4 2.7 2.0 73
A 313 3-13 3-15 0.5 0.7 4.5 670
316 3-23 4-1 0.3 0.2 4.1 2174
315 3-30 4-1 0.3 0.2 3.2 1327
318 4-59 1-17 0.3 4.6 4.0 86
257 3-13 1-5 0.4 3.1 3.2 104
283 3-13 1-5 0.4 5.4 3.7 69
637 3-13 1-5 0.4 4.3 3.0 70
638 3-13 1-5 0.4 4.1 3.3 82
B 624 3-23 1-17 0.3 5.0 3.9 79
284 3-30 1-17 0.3 4.6 3.4 75
653 3-33 1-17 0.3 4.3 0.3 7
268 4-34 1-27 0.3 5.5 3.8 69
633 4-34 1-27 0.6 6.9 3.0 44
730 3-7 1-5 0.3 1.1 2.8 249
728 3-7 1-5 0.3 2.0 3.2 157
691 3-9 3-20 0.3 2.8 3.1 109
749 3-33 3-15 0.3 3.8 2.3 62
750 3-33 1-16 0.3 3.0 2.8 92
724 3-33 1-17 0.3 2.3 3.4 151
706 3-33 1-16 0.3 3.6 3.0 84
C 744 1-18 1-12 0.4 5.1 3.0 59
696 3-11 1-16 0.4 3.0 2.9 97
685 3-13 3-20 0.3 0.5 3.4 734
732 3-15 1-17 0.3 4.5 3.2 72
694 3-15 1-5 0.4 5.2 2.9 55
743 3-23 1-12 0.3 3.2 0.3 10
742 3-23 2-28 0.4 4.2 3.1 74
693 3-23 1-12 0.5 4.2 4.0 94
136 3-23 2-28 0.4 5.0 2.7 55
155 3-30 1-16 0.4 1.0 2.2 221
163 3-30 1-16 0.3 0.6 3.0 506
171 3-30 1-16 0.3 1.0 2.8 295
145 3-43 1-5 0.4 4.4 2.9 65
49 3-48 3-11 0.3 1.7 2.6 155
51 3-48 1-39 0.1 1.9 0.1 4
159 3-7 6-21 0.4 3.9 3.6 92
169 3-7 6-21 0.3 1.3 3.1 235
134 3-9 1-5 0.4 5.0 2.9 58
141 4-31 1-33 2.4 4.2 2.6 63
142 4-31 1-33 0.4 4.2 2.8 67
The results obtained from these experiments demonstrate that somatically
mutated, high affinity heavy chains from different gene families are able to pair with
rearranged human germline V 1-39J 5 and V 3-20J 1 regions and be secreted from the
cell as a normal antibody molecule. As shown in Table 1, antibody titer was increased for
about 61% (42 of 69) heavy chains when paired with the rearranged human V 1-39J 5 light
chain and about 29% (20 of 69) heavy chains when paired with the rearranged human V 3-
20J 1 light chain as compared to the cognate light chain of the parental antibody. For about
% (14 of 69) of the heavy chains, both rearranged human germline light chains conferred
an increase in expression as compared to the cognate light chain of the parental antibody.
As shown in Table 2, the rearranged human germline V 1-39J 5 region conferred an
increase in expression of several heavy chains specific for a range of different classes of
antigens as compared to the cognate light chain for the parental antibodies. Antibody titer
was increased by more than two-fold for about 35% (15/43) of the heavy chains as
compared to the cognate light chain of the parental antibodies. For two heavy chains (315
and 316), the increase was greater than ten-fold as compared to the parental antibody.
Within all the heavy chains that showed increase expression relative to the cognate light
chain of the parental antibody, family three (V 3) heavy chains are over represented in
comparison to other heavy chain variable region gene families. This demonstrates a
favorable relationship of human V 3 heavy chains to pair with rearranged human germline
V 1-39J 5 and V 3-20J 1 light chains.
Example 2. Generation of a Rearranged Human Germline Light Chain Locus
Various rearranged human germline light chain targeting vectors were made
using VELOCIGENE® technology (see, e.g., US Pat. No. 6,586,251 and Valenzuela et al.
(2003) High-throughput engineering of the mouse genome coupled with high-resolution
expression analysis, Nature Biotech. 21(6): 652-659) to modify mouse genomic Bacterial
Artificial Chromosome (BAC) clones 302g12 and 254m04 (Invitrogen). Using these two BAC
clones, genomic constructs were engineered to contain a single rearranged human germline
light chain region and inserted into an endogenous light chain locus that was previously
modified to delete the endogenous variable and joining gene segments.
Construction of Rearranged Human Germline Light Chain Targeting
Vectors. Three different rearranged human germline light chain regions were made using
standard molecular biology techniques recognized in the art. The human variable gene
segments used for constructing these three regions included rearranged human V 1-39J 5
sequence, a rearranged human V 3-20J 1 sequence and a rearranged human VpreBJ 5
sequence.
A DNA segment containing exon 1 (encoding the leader peptide) and intron 1 of
the mouse V 3-7 gene was made by de novo DNA synthesis (Integrated DNA
Technologies). Part of the 5’ untranslated region up to a naturally occurring BlpI restriction
enzyme site was included. Exons of human V 1-39 and V 3-20 genes were PCR amplified
from human genomic BAC libraries. The forward primers had a 5’ extension containing the
splice acceptor site of intron 1 of the mouse V 3-7 gene. The reverse primer used for PCR
of the human V 1-39 sequence included an extension encoding human J 5, whereas the
reverse primer used for PCR of the human V 3-20 sequence included an extension
encoding human J 1. The human VpreBJ 5 sequence was made by de novo DNA
synthesis (Integrated DNA Technologies). A portion of the human J -C intron including the
splice donor site was PCR amplified from plasmid pBSHA18-PISceI. The forward PCR
primer included an extension encoding part of either a human J 5, J 1, or J 5 sequence.
The reverse primer included a PI-SceI site, which was previously engineered into the intron.
The mouse V 3-7 exon1/intron 1, human variable light chain exons, and human
J-C intron fragments were sewn together by overlap extension PCR, digested with BlpI
and PI-SceI, and ligated into plasmid pBSHA18-PISceI, which contained the promoter
from the human V 3-15 variable gene segment. A loxed hygromycin cassette within plasmid
pBSHA18-PISceI was replaced with a FRTed hygromycin cassette flanked by NotI and
AscI sites. The NotI/PI-SceI fragment of this plasmid was ligated into modified mouse BAC
254m04, which contained part of the mouse J -C intron, the mouse C exon, and about 75
kb of genomic sequence downstream of the mouse locus, which provided a 3’ homology
arm for homologous recombination in mouse ES cells. The NotI/AscI fragment of this BAC
was then ligated into modified mouse BAC 302g12, which contained a FRTed neomycin
cassette and about 23 kb of genomic sequence upstream of the endogenous locus for
homologous recombination in mouse ES cells.
Rearranged Human Germline V 1-39J 5 Targeting Vector (.
Restriction enzyme sites were introduced at the 5’ and 3’ ends of an engineered light chain
insert for cloning into a targeting vector: an AscI site at the 5’ end and a PI-SceI site at the 3’
end. Within the 5’ AscI site and the 3’ PI-SceI site the targeting construct from 5’ to 3’
included a 5’ homology arm containing sequence 5’ to the endogenous mouse light chain
locus obtained from mouse BAC clone 302g12, a FRTed neomycin resistance gene, an
genomic sequence including the human V 3-15 promoter, a leader sequence of the mouse
V 3-7 variable gene segment, a intron sequence of the mouse V 3-7 variable gene
segment, an open reading frame of a rearranged human germline V 1-39J 5 region, a
genomic sequence containing a portion of the human J -C intron, and a 3’ homology arm
containing sequence 3’ of the endogenous mouse J 5 gene segment obtained from mouse
BAC clone 254m04 (Figure 1, middle). Genes and/or sequences upstream of the
endogenous mouse light chain locus and downstream of the most 3’ J gene segment
(e.g., the endogenous 3’ enhancer) were unmodified by the targeting construct (see Figure
1). The sequence of the engineered human V 1-39J 5 locus is shown in SEQ ID NO: 1.
Targeted insertion of the rearranged human germline V 1-39J 5 region into BAC
DNA was confirmed by polymerase chain reaction (PCR) using primers located at
sequences within the rearranged human germline light chain region. Briefly, the intron
sequence 3’ to the mouse V 3-7 leader sequence was confirmed with primers ULC-m1F
(AGGTGAGGGT ACAGATAAGT GTTATGAG; SEQ ID NO: 2) and ULC-m1R
(TGACAAATGC CCTAATTATA GTGATCA; SEQ ID NO: 3). The open reading frame of the
rearranged human germline V 1-39J 5 region was confirmed with primers 1633-h2F
(GGGCAAGTCA GAGCATTAGC A; SEQ ID NO: 4) and 1633-h2R (TGCAAACTGG
ATGCAGCATA G; SEQ ID NO: 5). The neomycin cassette was confirmed with primers
neoF (GGTGGAGAGG CTATTCGGC; SEQ ID NO: 6) and neoR (GAACACGGCG
GCATCAG; SEQ ID NO: 7). Targeted BAC DNA was then used to electroporate mouse ES
cells to created modified ES cells for generating chimeric mice that express a rearranged
human germline V 1-39J 5 region.
Positive ES cell clones were confirmed by TAQMAN™ screening and karyotyping
using probes specific for the engineered V 1-39J 5 light chain region inserted into the
endogenous locus. Briefly, probe neoP (TGGGCACAAC AGACAATCGG CTG; SEQ ID NO:
8) which binds within the neomycin marker gene, probe ULC-m1P (CCATTATGAT
GCTCCATGCC TCTCTGTTC; SEQ ID NO: 9) which binds within the intron sequence 3’ to
the mouse V 3-7 leader sequence, and probe 1633h2P (ATCAGCAGAA ACCAGGGAAA
GCCCCT; SEQ ID NO: 10) which binds within the rearranged human germline V 1-39J 5
open reading frame. Positive ES cell clones were then used to implant female mice to give
rise to a litter of pups expressing the germline V 1-39J 5 light chain region.
Alternatively, ES cells bearing the rearranged human germline V 1-39J 5 light
chain region are transfected with a construct that expresses FLP in order to remove the
FRTed neomycin cassette introduced by the targeting construct. Optionally, the neomycin
cassette is removed by breeding to mice that express FLP recombinase (e.g., US
6,774,279). Optionally, the neomycin cassette is retained in the mice.
Rearranged Human Germline V 3-20J 1 Targeting Vector (. In a
similar fashion, an engineered light chain locus expressing a rearranged human germline
V 3-20J 1 region was made using a targeting construct including, from 5’ to 3’, a 5’
homology arm containing sequence 5’ to the endogenous mouse light chain locus obtained
from mouse BAC clone 302g12, a FRTed neomycin resistance gene, a genomic sequence
including the human V 3-15 promoter, a leader sequence of the mouse V 3-7 variable gene
segment, an intron sequence of the mouse V 3-7 variable gene segment, an open reading
frame of a rearranged human germline V 3-20J 1 region, a genomic sequence containing a
portion of the human J -C intron, and a 3’ homology arm containing sequence 3’ of the
endogenous mouse J 5 gene segment obtained from mouse BAC clone 254m04 (Figure 2,
middle). The sequence of the engineered human V 3-20J 1 locus is shown in SEQ ID NO:
Targeted insertion of the rearranged human germline V 3-20J 1 region into BAC
DNA was confirmed by polymerase chain reaction (PCR) using primers located at
sequences within the rearranged human germline V 3-20J 1 light chain region. Briefly, the
intron sequence 3’ to the mouse V 3-7 leader sequence was confirmed with primers ULC-
m1F (SEQ ID NO: 2) and ULC-m1R (SEQ ID NO: 3). The open reading frame of the
rearranged human germline V 3-20J 1 region was confirmed with primers 1635-h2F
(TCCAGGCACC CTGTCTTTG; SEQ ID NO: 12) and 1635-h2R (AAGTAGCTGC
TGCTAACACT CTGACT; SEQ ID NO: 13). The neomycin cassette was confirmed with
primers neoF (SEQ ID NO: 6) and neoR (SEQ ID NO: 7). Targeted BAC DNA was then
used to electroporate mouse ES cells to created modified ES cells for generating chimeric
mice that express the rearranged human germline V 3-20J 1 light chain.
Positive ES cell clones were confirmed by TAQMAN™ screening and karyotyping
using probes specific for the engineered V 3-20J 1 light chain region inserted into the
endogenous light chain locus. Briefly, probe neoP (SEQ ID NO: 8) which binds within the
neomycin marker gene, probe ULC-m1P (SEQ ID NO: 9) which binds within the mouse V 3-
7 leader sequence, and probe 1635h2P (AAAGAGCCAC CCTCTCCTGC AGGG; SEQ ID
NO: 14) which binds within the human V 3-20J 1 open reading frame. Positive ES cell
clones were then used to implant female mice. A litter of pups expressing the human
germline V 3-20J 1 light chain region.
Alternatively, ES cells bearing human germline V 3-20J 1 light chain region can
be transfected with a construct that expresses FLP in order to remove the FRTed neomycin
cassette introduced by the targeting construct. Optionally, the neomycin cassette may be
removed by breeding to mice that express FLP recombinase (e.g., US 6,774,279).
Optionally, the neomycin cassette is retained in the mice.
Rearranged Human Germline VpreBJ 5 Targeting Vector (. In a
similar fashion, an engineered light chain locus expressing a rearranged human germline
VpreBJ 5 region was made using a targeting construct including, from 5’ to 3’, a 5’
homology arm containing sequence 5’ to the endogenous mouse light chain locus obtained
from mouse BAC clone 302g12, a FRTed neomycin resistance gene, an genomic sequence
including the human V 3-15 promoter, a leader sequence of the mouse V 3-7 variable gene
segment, an intron sequence of the mouse V 3-7 variable gene segment, an open reading
frame of a rearranged human germline VpreBJ 5 region, a genomic sequence containing a
portion of the human J -C intron, and a 3’ homology arm containing sequence 3’ of the
endogenous mouse J 5 gene segment obtained from mouse BAC clone 254m04 (Figure 3,
middle). The sequence of the engineered human VpreBJ 5 locus is shown in SEQ ID NO:
Targeted insertion of the rearranged human germline VpreBJ 5 region into BAC
DNA was confirmed by polymerase chain reaction (PCR) using primers located at
sequences within the rearranged human germline VpreBJ 5 region light chain region.
Briefly, the intron sequence 3’ to the mouse V 3-7 leader sequence was confirmed with
primers ULC-m1F (SEQ ID NO: 2) and ULC-m1R (SEQ ID NO: 3). The open reading frame
of the rearranged human germline VpreBJ 5 region was confirmed with primers 1616-h1F
(TGTCCTCGGC CCTTGGA; SEQ ID NO: 16) and 1616-h1R (CCGATGTCAT
GGTCGTTCCT; SEQ ID NO: 17). The neomycin cassette was confirmed with primers neoF
(SEQ ID NO: 6) and neoR (SEQ ID NO: 7). Targeted BAC DNA was then used to
electroporate mouse ES cells to created modified ES cells for generating chimeric mice that
express the rearranged human germline VpreBJ 5 light chain.
Positive ES cell clones are confirmed by TAQMAN™ screening and karyotyping
using probes specific for the engineered VpreBJ 5 light chain region inserted into the
endogenous light chain locus. Briefly, probe neoP (SEQ ID NO:8), which binds within the
neomycin marker gene, probe ULC-m1P (SEQ ID NO: 9), which binds within the mouse
IgV 3-7 leader sequence, and probe 1616h1P (ACAATCCGCC TCACCTGCAC CCT; SEQ
ID NO: 18) which binds within the human VpreBJ 5 open reading frame. Positive ES cell
clones are then used to implant female mice to give rise to a litter of pups expressing a
germline light chain region.
Alternatively, ES cells bearing the rearranged human germline VpreBJ 5 light
chain region are transfected with a construct that expresses FLP in order to remove the
FRTed neomycin cassette introduced by the targeting construct. Optionally, the neomycin
cassette is removed by breeding to mice that express FLP recombinase (e.g., US
6,774,279). Optionally, the neomycin cassette is retained in the mice.
Example 3. Generation of Mice Expressing a Single Rearranged Human Light Chain
Targeted ES cells described above were used as donor ES cells and introduced
into an 8-cell stage mouse embryo by the VELOCIMOUSE® method (see, e.g., US Pat. No.
7,294,754 and Poueymirou et al. (2007) F0 generation mice that are essentially fully derived
from the donor gene-targeted ES cells allowing immediate phenotypic analyses Nature
Biotech. 25(1): 91-99. VELOCIMICE® independently bearing an engineered human
germline V 1-39J 5 light chain region, a V 3-20J 1 light chain region or a VpreBJ 5 light
chain region are identified by genotyping using a modification of allele assay (Valenzuela et
al., supra) that detects the presence of the unique rearranged human germline light chain
region.
Pups are genotyped and a pup heterozygous or homozygous for the unique
rearranged human germline light chain region are selected for characterizing expression of
the rearranged human germline light chain region.
Flow Cytometry. Expression of the rearranged human light chain region in the
normal antibody repertoire of common light chain mice was validated by analysis of
immunoglobulin and expression in splenocytes and peripheral blood of common light
chain mice. Cell suspensions from harvested spleens and peripheral blood of wild type
(n=5), V 1-39J 5 common light chain heterozygote (n=3), V 1-39J 5 common light chain
homozygote (n=3), V 3-20J 1 common light chain heterozygote (n=2), and V 3-20J 1
common light chain homozygote (n=2) mice were made using standard methods and stained
+ + +
with CD19 , Ig and Ig using fluorescently labeled antibodies (BD Pharmigen).
Briefly, 1x10 cells were incubated with anti-mouse CD16/CD32 (clone 2.4G2, BD
Pharmigen) on ice for 10 minutes, followed by labeling with the following antibody cocktail for
minutes on ice: APC conjugated anti-mouse CD19 (clone 1D3, BD Pharmigen), PerCP-
Cy5.5 conjugated anti-mouse CD3 (clone 17A2, BioLegend), FITC conjugated anti-mouse
Ig (clone 187.1, BD Pharmigen), PE conjugated anti-mouse Ig (clone RML-42,
BioLegend). Following staining, cells were washed and fixed in 2% formaldehyde. Data
acquisition was performed on an LSRII flow cytometer and analyzed with FlowJo. Gating:
+ - + + - + - + - + + -
total B cells (CD19 CD3 ), Ig B cells (Ig Ig CD19 CD3 ), Ig B cells (Ig Ig CD19 CD3
). Data gathered from blood and splenocyte samples demonstrated similar results. Table 3
sets forth the percent positive CD19 B cells from peripheral blood of one representative
+ + + + +
mouse from each group that are Ig , Ig , or Ig Ig . Percent of CD19 B cells in
peripheral blood from wild type (WT) and mice homozygous for either the V 1-39J 5 or V 3-
20J 1 common light chain are shown in
TABLE 3
CD19 B cells
Mouse
+ + + +
Ig Ig Ig Ig
Wild type 4.8 93 0.53
V 1-39J 5 1.4 93 2.6
V 3-20J 1 4.2 88 6
Common Light Chain Expression. Expression of each common light chain
(V 1-39J 5 and V 3-20J 1) was analyzed in heterozygous and homozygous mice using a
quantitative PCR assay (e.g. TAQMAN ).
Briefly, CD19 B cells were purified from the spleens of wild type, mice
homozygous for a replacement of the mouse heavy chain and light chain variable region
loci with corresponding human heavy chain and light chain variable region loci (H ), as
well as mice homozygous and heterozygous for each rearranged human light chain region
(V 1-39J 5 or V 3-20J 1) using mouse CD19 Microbeads (Miltenyi Biotec) according to
manufacturer’s specifications. Total RNA was purified from CD19 B cells using RNeasy
Mini kit (Qiagen) according to manufacturer’s specifications and genomic RNA was removed
using an RNase-free DNase on-column treatment (Qiagen). 200 ng mRNA was reverse-
transcribed into cDNA using the First Stand cDNA Synthesis kit (Invitrogen) and the resulting
cDNA was amplified with the Taqman Universal PCR Master Mix (Applied Biosystems). All
reactions were performed using the ABI 7900 Sequence Detection System (Applied
Biosystems) using primers and Taqman MGB probes spanning (1) the V -J junction for
both common light chains, (2) the V gene alone (i.e. V 1-39 and V 3-20), and (3) the
mouse C region. Table 4 sets forth the sequences of the primers and probes employed for
this assay. Relative expression was normalized to expression of the mouse C region.
Results are shown in , 5B and 5C.
TABLE 4
Region Primer/Probe Description (5’-3’) SEQ ID NOs:
(Sense) AGCAGTCTGC AACCTGAAGA TTT 19
V 1-39J 5 Junction (Anti-sense) GTTTAATCTC CAGTCGTGTC CCTT 20
(Probe) CCTCCGATCA CCTTC 21
(Sense) AAACCAGGGA AAGCCCCTAA 22
V 1-39 (Anti-sense) ATGGGACCCC ACTTTGCA 23
(Probe) CTCCTGATCT ATGCTGCAT 24
(Sense) CAGCAGACTG GAGCCTGAAG A 25
V 3-20J 1 Junction (Anti-sense) TGATTTCCAC CTTGGTCCCT T 26
(Probe) TAGCTCACCT TGGACGTT 27
(Sense) CTCCTCATCT ATGGTGCATC CA 28
V 3-20 (Anti-sense) GACCCACTGC CACTGAACCT 29
(Probe) CCACTGGCAT CCC 30
(Sense) TGAGCAGCAC CCTCACGTT 31
Mouse C (Anti-sense) GTGGCCTCAC AGGTATAGCT GTT 32
(Probe) ACCAAGGACG AGTATGAA 33
Antigen Specific Common Light Chain Antibodies. Common light chain mice
bearing either a V 1-39J 5 or V 3-20J 1 common light chain at the endogenous mouse
light chain locus were immunized with -galactosidase and antibody titer was measured.
Briefly, -galactosidase (Sigma) was emulsified in titermax adjuvant (Sigma), as
per manufacturer’s directions. Wild type (n=7), V 1-39J 5 common light chain homozygotes
(n=2) and V 3-20J 1 common light chain homozygotes (n=5) were immunized by
subcutaneous injection with 100 µg -galactosidase/Titermax. Mice were boosted by
subcutaneous injection two times, 3 weeks apart, with 50 µg -galactosidase/Titermax. After
the second boost, blood was collected from anaesthetized mice using a retro-orbital bleed
into serum separator tubes (BD Biosciences) as per manufacturer’s directions. To measure
anti- -galactosidase IgM or IgG antibodies, ELISA plates (Nunc) were coated with 1 µg/mL
-galactosidase overnight at 4 C. Excess antigen was washed off before blocking with PBS
with 1% BSA for one hour at room temperature. Serial dilutions of serum were added to the
plates and incubated for one hour at room temperature before washing. Plates were then
incubated with HRP conjugated anti-IgM (Southern Biotech) or anti-IgG (Southern Biotech)
for one hour at room temperature. Following another wash, plates were developed with
TMB substrate (BD Biosciences). Reactions were stopped with 1N sulfuric acid and OD
was read using a Victor X5 Plate Reader (Perkin Elmer). Data was analyzed with GraphPad
Prism and signal was calculated as the dilution of serum that is two times above
background. Results are shown in and 6B.
As shown in this Example, the ratio of / B cells in both the splenic and
peripheral compartments of V 1-39J 5 and V 3-20J 1 common light chain mice
demonstrated a near wild type pattern (Table 3 and . VpreBJ 5 common light chain
mice, however, demonstrated fewer peripheral B cells, of which about 1-2% express the
engineered human light chain region (data not shown). The expression levels of the V 1-
39J 5 and V 3-20J 1 rearranged human light chain regions from the endogenous light
chain locus were elevated in comparison to an endogenous light chain locus containing a
complete replacement of mouse V and J gene segments with human V and J gene
segments (, 5B and 5C). The expression levels of the VpreBJ 5 rearranged human
light chain region demonstrated similar high expression from the endogenous light chain
locus in both heterozygous and homozygous mice (data not shown). This demonstrates that
in direct competition with the mouse , , or both endogenous light chain loci, a single
rearranged human V /J sequence can yield better than wild type level expression from the
endogenous light chain locus and give rise to normal splenic and blood B cell frequency.
Further, the presence of an engineered light chain locus having either a human V 1-39J 5
or human V 3-20J 1 sequence was well tolerated by the mice and appear to function in wild
type fashion by representing a substantial portion of the light chain repertoire in the humoral
component of the immune response (FIG 6A and 6B).
Example 4. Breeding of Mice Expressing a Single Rearranged Human Germline Light
Chain
This Example describes several other genetically modified mouse strains that can
be bred to any one of the common light chain mice described herein to create multiple
genetically modified mouse strains harboring multiple genetically modified immunoglobulin
loci.
Endogenous Ig Knockout (KO). To optimize the usage of the engineered light
chain locus, mice bearing one of the rearranged human germline light chain regions are bred
to another mouse containing a deletion in the endogenous light chain locus. In this
manner, the progeny obtained will express, as their only light chain, the rearranged human
germline light chain region as described in Example 2. Breeding is performed by standard
techniques recognized in the art and, alternatively, by a commercial breeder (e.g., The
Jackson Laboratory). Mouse strains bearing an engineered light chain locus and a deletion
of the endogenous light chain locus are screened for presence of the unique light chain
region and absence of endogenous mouse light chains.
Humanized Endogenous Heavy Chain Locus. Mice bearing an engineered
human germline light chain locus are bred with mice that contain a replacement of the
endogenous mouse heavy chain variable gene locus with the human heavy chain variable
gene locus (see US 6,596,541; the VELOCIMMUNE® mouse, Regeneron Pharmaceuticals,
Inc.). The VELOCIMMUNE® mouse comprises a genome comprising human heavy chain
variable regions operably linked to endogenous mouse constant region loci such that the
mouse produces antibodies comprising a human heavy chain variable region and a mouse
heavy chain constant region in response to antigenic stimulation. The DNA encoding the
variable regions of the heavy chains of the antibodies is isolated and operably linked to DNA
encoding the human heavy chain constant regions. The DNA is then expressed in a cell
capable of expressing the fully human heavy chain of the antibody.
Mice bearing a replacement of the endogenous mouse V locus with the human
VH locus and a single rearranged human germline V region at the endogenous light chain
locus are obtained. Reverse chimeric antibodies containing somatically mutated heavy
chains (human V and mouse C ) with a single human light chain (human V and mouse C )
H H L L
are obtained upon immunization with an antigen of interest. V and V nucleotide
sequences of B cells expressing the antibodies are identified and fully human antibodies are
made by fusion the V and V nucleotide sequences to human C and C nucleotide
H L H L
sequences in a suitable expression system.
Example 5. Generation of Antibodies from Mice Expressing Human Heavy Chains and
a Rearranged Human Germline Light Chain Region
After breeding mice that contain the engineered human light chain region to
various desired strains containing modifications and deletions of other endogenous Ig loci
(as described in Example 4), selected mice can be immunized with an antigen of interest.
Generally, a VELOCIMMUNE® mouse containing one of the single rearranged
human germline light chain regions is challenged with an antigen, and lymphatic cells (such
as B-cells) are recovered from serum of the animals. The lymphatic cells are fused with a
myeloma cell line to prepare immortal hybridoma cell lines, and such hybridoma cell lines
are screened and selected to identify hybridoma cell lines that produce antibodies containing
human heavy chain variables and a rearranged human germline light chains which are
specific to the antigen used for immunization. DNA encoding the variable regions of the
heavy chains and the light chain are isolated and linked to desirable isotypic constant
regions of the heavy chain and light chain. Due to the presence of the endogenous mouse
sequences and any additional cis-acting elements present in the endogenous locus, the
single light chain of each antibody may be somatically mutated. This adds additional
diversity to the antigen-specific repertoire comprising a single light chain and diverse heavy
chain sequences. The resulting cloned antibody sequences are subsequently expressed in
a cell, such as a CHO cell. Alternatively, DNA encoding the antigen-specific chimeric
antibodies or the variable domains of the light and heavy chains is identified directly from
antigen-specific lymphocytes.
Initially, high affinity chimeric antibodies are isolated having a human variable
region and a mouse constant region. As described above, the antibodies are characterized
and selected for desirable characteristics, including affinity, selectivity, epitope, etc. The
mouse constant regions are replaced with a desired human constant region to generate the
fully human antibody containing a somatically mutated human heavy chain and a single light
chain derived from a rearranged human germline light chain region of the invention. Suitable
human constant regions include, for example wild type or modified IgG1 or IgG4.
Separate cohorts of VELOCIMMUNE® mice containing a replacement of the
endogenous mouse heavy chain locus with human V , D , and J gene segments and a
H H H
replacement of the endogenous mouse light chain locus with either the engineered
germline V 1-39J 5 human light chain region or the engineered germline V 3-20J 1 human
light chain region (described above) were immunized with a human cell-surface receptor
protein (Antigen E). Antigen E is administered directly onto the hind footpad of mice with six
consecutive injections every 3-4 days. Two to three micrograms of Antigen E are mixed with
µg of CpG oligonucleotide (Cat # tlrl-modn - ODN1826 oligonucleotide; InVivogen, San
Diego, CA) and 25 µg of Adju-Phos (Aluminum phosphate gel adjuvant, Cat# H250;
Brenntag Biosector, Frederikssund, Denmark) prior to injection. A total of six injections are
given prior to the final antigen recall, which is given 3-5 days prior to sacrifice. Bleeds after
the 4th and 6th injection are collected and the antibody immune response is monitored by a
standard antigen-specific immunoassay.
When a desired immune response is achieved splenocytes are harvested and
fused with mouse myeloma cells to preserve their viability and form hybridoma cell lines.
The hybridoma cell lines are screened and selected to identify cell lines that produce Antigen
E-specific common light chain antibodies. Using this technique several anti-Antigen E-
specific common light chain antibodies (i.e., antibodies possessing human heavy chain
variable domains, the same human light chain variable domain, and mouse constant
domains) are obtained.
Alternatively, anti-Antigen E common light chain antibodies are isolated directly
from antigen-positive B cells without fusion to myeloma cells, as described in U.S.
2007/0280945A1, herein specifically incorporated by reference in its entirety. Using this
method, several fully human anti-Antigen E common light chain antibodies (i.e., antibodies
possessing human heavy chain variable domains, either an engineered human V 1-39J 5
light chain or an engineered human V 3-20J 1 light chain region, and human constant
domains) were obtained.
The biological properties of the exemplary anti-Antigen E common light chain
antibodies generated in accordance with the methods of this Example are described in detail
in the sections set forth below.
Example 6. Heavy Chain Gene Segment Usage in Antigen-Specific Common Light
Chain Antibodies
To analyze the structure of the human anti-Antigen E common light chain
antibodies produced, nucleic acids encoding heavy chain antibody variable regions were
cloned and sequenced. From the nucleic acid sequences and predicted amino acid
sequences of the antibodies, gene usage was identified for the heavy chain variable region
(HCVR) of selected common light chain antibodies obtained from immunized
VELOCIMMUNE® mice containing either the engineered human V 1-39J 5 light chain or
engineered human V 3-20J 1 light chain region. Results are shown in Tables 5 and 6,
which demonstrate that mice according to the invention generate antigen-specific common
light chain antibodies from a variety of human heavy chain gene segments, due to a variety
of rearrangements, when employing either a mouse that expresses a light chain from only a
human V 1 or a human V 3derived light chain. Human V gene segments of the 2,
3, 4, and 5 families rearranged with a variety of human D segments and human J
segments to yield antigen-specific antibodies.
TABLE 5
V 1-39J 5
Common Light Chain Antibodies
HCVR HCVR
Antibody Antibody
V D J V D J
H H H H H H
2952 2-5 6-6 1 6030 3-30 6-6 5
5978 2-5 6-6 1 6032 3-30 6-6 5
5981 2-5 3-22 1 2985 3-30 6-13 4
6027 3-13 6-6 5 2997 3-30 6-13 4
3022 3-23 3-10 4 3011 3-30 6-13 4
3028 3-23 3-3 4 3047 3-30 6-13 4
5999 3-23 6-6 4 5982 3-30 6-13 4
6009 3-23 2-8 4 6002 3-30 6-13 4
6011 3-23 7-27 4 6003 3-30 6-13 4
5980 3-30 1-1 4 6012 3-30 6-13 4
3014 3-30 1-7 4 6013 3-30 6-13 4
3015 3-30 1-7 4 6014 3-30 6-13 4
3023 3-30 1-7 4 6015 3-30 6-13 4
3024 3-30 1-7 4 6016 3-30 6-13 4
3032 3-30 1-7 4 6017 3-30 6-13 4
6024 3-30 1-7 4 6020 3-30 6-13 4
6025 3-30 1-7 4 6034 3-30 6-13 4
6031 3-30 1-7 4 2948 3-30 7-27 4
6007 3-30 3-3 4 2987 3-30 7-27 4
2982 3-30 3-22 5 2996 3-30 7-27 4
6001 3-30 3-22 5 3005 3-30 7-27 4
6005 3-30 3-22 5 3012 3-30 7-27 4
6035 3-30 5-5 2 3020 3-30 7-27 4
3013 3-30 5-12 4 3021 3-30 7-27 4
3042 3-30 5-12 4 3025 3-30 7-27 4
2955 3-30 6-6 1 3030 3-30 7-27 4
3043 3-30 6-6 3 3036 3-30 7-27 4
3018 3-30 6-6 4 5997 3-30 7-27 4
2949 3-30 6-6 5 6033 3-30 7-27 4
2950 3-30 6-6 5 3004 3-30 7-27 5
2954 3-30 6-6 5 6028 3-30 7-27 6
2978 3-30 6-6 5 3010 4-59 3-16 3
3016 3-30 6-6 5 3019 4-59 3-16 3
3017 3-30 6-6 5 6018 4-59 3-16 3
3033 3-30 6-6 5 6026 4-59 3-16 3
3041 3-30 6-6 5 6029 4-59 3-16 3
5979 3-30 6-6 5 6036 4-59 3-16 3
5998 3-30 6-6 5 6037 4-59 3-16 3
6004 3-30 6-6 5 2964 4-59 3-22 3
6010 3-30 6-6 5 3027 4-59 3-16 4
6019 3-30 6-6 5 3046 5-51 5-5 3
6021 3-30 6-6 5 6000 1-69 6-13 4
6022 3-30 6-6 5 6006 1-69 6-6 5
6023 3-30 6-6 5 6008 1-69 6-13 4
TABLE 6
V 3-20J 1
Common Light Chain Antibodies
HCVR HCVR
Antibody Antibody
V D J V D J
H H H H H H
5989 3-30 3-3 3 5992 4-39 1-26 3
5994 3-33 1-7 4 2975 5-51 6-13 5
5985 3-33 2-15 4 2972 5-51 3-16 6
5987 3-33 2-15 4 5986 5-51 3-16 6
5995 3-33 2-15 4 5993 5-51 3-16 6
2968 4-39 1-26 3 5996 5-51 3-16 6
5988 4-39 1-26 3 5984 3-53 1-1 4
5990 4-39 1-26 3
Example 7. Determination of Blocking Ability of Antigen-Specific Common Light
Chain Antibodies by LUMINEX™ Assay
Ninety-eight human common light chain antibodies raised against Antigen E were
tested for their ability to block binding of Antigen E’s natural ligand (Ligand Y) to Antigen E in
a bead-based assay.
The extracellular domain (ECD) of Antigen E was conjugated to two myc epitope
tags and a 6X histidine tag (Antigen E-mmH) and amine-coupled to carboxylated
microspheres at a concentration of 20 µg/mL in MES buffer. The mixture was incubated for
two hours at room temperature followed by bead deactivation with 1M Tris pH 8.0 followed
by washing in PBS with 0.05% (v/v) Tween-20. The beads were then blocked with PBS
(Irvine Scientific, Santa Ana, CA) containing 2% (w/v) BSA (Sigma-Aldrich Corp., St. Louis,
MO). In a 96-well filter plate, supernatants containing Antigen E-specific common light chain
antibodies were diluted 1:15 in buffer. A negative control containing a mock supernatant
with the same media components as for the antibody supernatant was prepared. Antigen E-
labeled beads were added to the supernatants and incubated overnight at 4°C. Biotinylated-
Ligand Y protein was added to a final concentration of 0.06 nM and incubated for two hours
at room temperature. Detection of biotinylated-Ligand Y bound to Antigen E-myc-myc-6His
labeled beads was determined with R-Phycoerythrin conjugated to Streptavidin (Moss Inc,
Pasadena, MD) followed by measurement in a LUMINEX™ flow cytometry-based analyzer.
Background Mean Fluorescence Intensity (MFI) of a sample without Ligand Y was
subtracted from all samples. Percent blocking was calculated by division of the background-
subtracted MFI of each sample by the adjusted negative control value, multiplying by 100
and subtracting the resulting value from 100.
In a similar experiment, the same 98 human common light chain antibodies
raised against Antigen E were tested for their ability to block binding of Antigen E to Ligand
Y-labeled beads.
Briefly, Ligand Y was amine-coupled to carboxylated microspheres at a
concentration of 20 µg/mL diluted in MES buffer. The mixture and incubated two hours at
room temperature followed by deactivation of beads with 1M Tris pH 8 then washing in PBS
with 0.05% (v/v) Tween-20. The beads were then blocked with PBS (Irvine Scientific, Santa
Ana, CA) containing 2% (w/v) BSA (Sigma-Aldrich Corp., St. Louis, MO). In a 96-well filter
plate, supernatants containing Antigen E-specific common light chain antibodies were diluted
1:15 in buffer. A negative control containing a mock supernatant with the same media
components as for the antibody supernatant was prepared. A biotinylated-Antigen E-mmH
was added to a final concentration of 0.42 nM and incubated overnight at 4°C. Ligand Y-
labeled beads were then added to the antibody/Antigen E mixture and incubated for two
hours at room temperature. Detection of biotinylated-Antigen E-mmH bound to Ligand Y-
beads was determined with R-Phycoerythrin conjugated to Streptavidin (Moss Inc,
Pasadena, MD) followed by measurement in a LUMINEX™ flow cytometry-based analyzer.
Background Mean Fluorescence Intensity (MFI) of a sample without Antigen E was
subtracted from all samples. Percent blocking was calculated by division of the background-
subtracted MFI of each sample by the adjusted negative control value, multiplying by 100
and subtracting the resulting value from 100.
Tables 7 and 8 show the percent blocking for all 98 anti-Antigen E common light
chain antibodies tested in both LUMINEX™ assays. ND: not determined under current
experimental conditions.
TABLE 7
V 1-39J 5
Common Light Chain Antibodies
% Blocking of % Blocking of
Antibody
Antigen E-Labeled Beads Antigen E In Solution
2948 81.1 47.8
2948G 38.6 ND
2949 97.6 78.8
2949G 97.1 73.7
2950 96.2 81.9
2950G 89.8 31.4
2952 96.1 74.3
2952G 93.5 39.9
2954 93.7 70.1
2954G 91.7 30.1
2955 75.8 30.0
2955G 71.8 ND
2964 92.1 31.4
2964G 94.6 43.0
2978 98.0 95.1
2978G 13.9 94.1
2982 92.8 78.5
2982G 41.9 52.4
2985 39.5 31.2
2985G 2.0 5.0
2987 81.7 67.8
2987G 26.6 29.3
2996 87.3 55.3
2996G 95.9 38.4
2997 93.4 70.6
2997G 9.7 7.5
3004 79.0 48.4
3004G 60.3 40.7
3005 97.4 93.5
3005G 77.5 75.6
3010 98.0 82.6
3010G 97.9 81.0
3011 87.4 42.8
3011G 83.5 41.7
3012 91.0 60.8
3012G 52.4 16.8
3013 80.3 65.8
3013G 17.5 15.4
3014 63.4 20.7
3014G 74.4 28.5
3015 89.1 55.7
3015G 58.8 17.3
3016 97.1 81.6
3016G 93.1 66.4
3017 94.8 70.2
3017G 87.9 40.8
3018 85.4 54.0
3018G 26.1 12.7
3019 99.3 92.4
3019G 99.3 88.1
3020 96.7 90.3
3020G 85.2 41.5
3021 74.5 26.1
3021G 81.1 27.4
3022 65.2 17.6
3022G 67.2 9.1
3023 71.4 28.5
3023G 73.8 29.7
3024 73.9 32.6
3024G 89.0 10.0
3025 70.7 15.6
3025G 76.7 24.3
3027 96.2 61.6
3027G 98.6 75.3
3028 92.4 29.0
3028G 87.3 28.8
3030 6.0 10.6
3030G 41.3 14.2
3032 76.5 31.4
3032G 17.7 11.0
3033 98.2 86.1
3033G 93.6 64.0
3036 74.7 32.7
3036G 90.1 51.2
3041 95.3 75.9
3041G 92.4 51.6
3042 88.1 73.3
3042G 60.9 25.2
3043 90.8 65.8
3043G 92.8 60.3
TABLE 8
V 3-20J 1
Common Light Chain Antibodies
% Blocking of % Blocking of
Antibody
Antigen E-Labeled Beads Antigen E In Solution
2968 97.1 73.3
2968G 67.1 14.6
2969 51.7 20.3
2969G 37.2 16.5
2970 92.2 34.2
2970G 92.7 27.2
2971 23.4 11.6
2971G 18.8 18.9
2972 67.1 38.8
2972G 64.5 39.2
2973 77.7 27.0
2973G 51.1 20.7
2974 57.8 12.4
2974G 69.9 17.6
2975 49.4 18.2
2975G 32.0 19.5
2976 1.0 1.0
2976G 50.4 20.4
In the first LUMINEX™ experiment described above, 80 common light chain
antibodies containing the V 1-39J 5 engineered light chain were tested for their ability to
block Ligand Y binding to Antigen E-labeled beads. Of these 80 common light chain
antibodies, 68 demonstrated >50% blocking, while 12 demonstrated <50% blocking (6 at 25-
50% blocking and 6 at <25% blocking). For the 18 common light chain antibodies containing
the V 3-20J 1 engineered light chain, 12 demonstrated >50% blocking, while 6
demonstrated <50% blocking (3 at 25-50% blocking and 3 at <25% blocking) of Ligand Y
binding to Antigen E-labeled beads.
In the second LUMINEX™ experiment described above, the same 80 common
light chain antibodies containing the V 1-39J 5 engineered light chain were tested for their
ability to block binding of Antigen E to Ligand Y-labeled beads. Of these 80 common light
chain antibodies, 36 demonstrated >50% blocking, while 44 demonstrated <50% blocking
(27 at 25-50% blocking and 17 at <25% blocking). For the 18 common light chain antibodies
containing the V 3-20J 1 engineered light chain, 1 demonstrated >50% blocking, while 17
demonstrated <50% blocking (5 at 25-50% blocking and 12 at <25% blocking) of Antigen E
binding to Ligand Y-labeled beads.
The data of Tables 7 and 8 establish that the rearrangements described in Tables
and 6 generated anti-Antigen E-specific common light chain antibodies that blocked
binding of Ligand Y to its cognate receptor Antigen E with varying degrees of efficacy, which
is consistent with the anti-Antigen E common light chain antibodies of Tables 5 and 6
comprising antibodies with overlapping and non-overlapping epitope specificity with respect
to Antigen E.
Example 8. Determination of Blocking Ability of Antigen-Specific Common Light
Chain Antibodies by ELISA
Human common light chain antibodies raised against Antigen E were tested for
their ability to block Antigen E binding to a Ligand Y-coated surface in an ELISA assay.
Ligand Y was coated onto 96-well plates at a concentration of 2 µg/mL diluted in
PBS and incubated overnight followed by washing four times in PBS with 0.05% Tween-20.
The plate was then blocked with PBS (Irvine Scientific, Santa Ana, CA) containing 0.5%
(w/v) BSA (Sigma-Aldrich Corp., St. Louis, MO) for one hour at room temperature. In a
separate plate, supernatants containing anti-Antigen E common light chain antibodies were
diluted 1:10 in buffer. A mock supernatant with the same components of the antibodies was
used as a negative control. Antigen E-mmH (described above) was added to a final
concentration of 0.150 nM and incubated for one hour at room temperature. The
antibody/Antigen E-mmH mixture was then added to the plate containing Ligand Y and
incubated for one hour at room temperature. Detection of Antigen E-mmH bound to Ligand
Y was determined with Horse-Radish Peroxidase (HRP) conjugated to anti-Penta-His
antibody (Qiagen, Valencia, CA) and developed by standard colorimetric response using
tetramethylbenzidine (TMB) substrate (BD Biosciences, San Jose, CA) neutralized by
sulfuric acid. Absorbance was read at OD450 for 0.1 sec. Background absorbance of a
sample without Antigen E was subtracted from all samples. Percent blocking was calculated
by division of the background-subtracted MFI of each sample by the adjusted negative
control value, multiplying by 100 and subtracting the resulting value from 100.
Tables 9 and 10 show the percent blocking for all 98 anti-Antigen E common light
chain antibodies tested in the ELISA assay. ND: not determined under current experimental
conditions.
TABLE 9
V 1-39J 5
Common Light Chain Antibodies
% Blocking of % Blocking of
Antibody Antibody
Antigen E In Solution Antigen E In Solution
2948 21.8 3015 23.7
2948G 22.9 3015G 10.2
2949 79.5 3016 78.1
2949G 71.5 3016G 37.4
2950 80.4 3017 61.6
2950G 30.9 3017G 25.2
2952 66.9 3018 40.6
2952G 47.3 3018G 14.5
2954 55.9 3019 94.6
2954G 44.7 3019G 92.3
2955 12.1 3020 80.8
2955G 25.6 3020G ND
2964 34.8 3021 7.6
2964G 47.7 3021G 20.7
2978 90.0 3022 2.4
2978G 90.2 3022G 15.0
2982 59.0 3023 9.1
2982G 20.4 3023G 19.2
2985 10.5 3024 7.5
2985G ND 3024G 15.2
2987 31.4 3025 ND
2987G ND 3025G 13.9
2996 29.3 3027 61.4
2996G ND 3027G 82.7
2997 48.7 3028 40.3
2997G ND 3028G 12.3
3004 16.7 3030 ND
3004G 3.5 3030G 9.5
3005 87.2 3032 ND
3005G 54.3 3032G 13.1
3010 74.5 3033 77.1
3010G 84.6 3033G 32.9
3011 19.4 3036 17.6
3011G ND 3036G 24.6
3012 45.0 3041 59.3
3012G 12.6 3041G 30.7
3013 39.0 3042 39.9
3013G 9.6 3042G 16.1
3014 5.2 3043 57.4
3014G 17.1 3043G 46.1
TABLE 10
V 3-20J 1
Common Light Chain Antibodies
% Blocking of % Blocking of
Antibody Antibody
Antigen E In Solution Antigen E In Solution
2968 68.9 2972G 35.7
2968G 15.2 2973 20.7
2969 10.1 2973G 23.1
2969G 23.6 2974 ND
2970 34.3 2974G 22.0
2970G 41.3 2975 8.7
2971 6.3 2975G 19.2
2971G 27.1 2976 4.6
2972 9.6 2976G 26.7
As described in this Example, of the 80 common light chain antibodies containing
the V 1-39J 5 engineered light chain tested for their ability to block Antigen E binding to a
Ligand Y-coated surface, 22 demonstrated >50% blocking, while 58 demonstrated <50%
blocking (20 at 25-50% blocking and 38 at <25% blocking). For the 18 common light chain
antibodies containing the V 3-20J 1 engineered light chain, one demonstrated >50%
blocking, while 17 demonstrated <50% blocking (5 at 25-50% blocking and 12 at <25%
blocking) of Antigen E binding to a Ligand Y-coated surface.
These results are also consistent with the Antigen E-specific common light chain
antibody pool comprising antibodies with overlapping and non-overlapping epitope specificity
with respect to Antigen E.
Example 9. BIACORE™ Affinity Determination for Antigen-Specific Common Light
Chain Antibodies
Equilibrium dissociation constants (K ) for selected antibody supernatants were
determined by SPR (Surface Plasmon Resonance) using a BIACORE™ T100 instrument
(GE Healthcare). All data was obtained using HBS-EP (10mM Hepes, 150mM NaCl, 0.3mM
EDTA, 0.05% Surfactant P20, pH 7.4) as both the running and sample buffers, at 25°C.
Antibodies were captured from crude supernatant samples on a CM5 sensor chip surface
previously derivatized with a high density of anti-human Fc antibodies using standard amine
coupling chemistry. During the capture step, supernatants were injected across the anti-
human Fc surface at a flow rate of 3 µL/min, for a total of 3 minutes. The capture step was
followed by an injection of either running buffer or analyte at a concentration of 100 nM for 2
minutes at a flow rate of 35 µL/min. Dissociation of antigen from the captured antibody was
monitored for 6 minutes. The captured antibody was removed by a brief injection of 10 mM
glycine, pH 1.5. All sensorgrams were double referenced by subtracting sensorgrams from
buffer injections from the analyte sensorgrams, thereby removing artifacts caused by
dissociation of the antibody from the capture surface. Binding data for each antibody was fit
to a 1:1 binding model with mass transport using BIAcore T100 Evaluation software v2.1.
Results are shown in Tables 11 and 12.
TABLE 11
V 1-39J 5
Common Light Chain Antibodies
100 nM Antigen E 100 nM Antigen E
Antibody Antibody
K (nM) T (min) K (nM) T (min)
D 1/2 D 1/2
2948 8.83 28 3015 29.1 11
2948G 95.0 1 3015G 65.9 0
2949 3.57 18 3016 4.99 17
2949G 6.37 9 3016G 18.9 4
2950 4.91 17 3017 9.83 8
2950G 13.6 5 3017G 55.4 2
2952 6.25 7 3018 11.3 36
2952G 7.16 4 3018G 32.5 3
2954 2.37 24 3019 1.54 59
2954G 5.30 9 3019G 2.29 42
2955 14.4 6 3020 5.41 39
2955G 12.0 4 3020G 41.9 6
2964 14.8 6 3021 50.1 6
2964G 13.0 9 3021G 26.8 4
2978 1.91 49 3022 25.7 17
2978G 1.80 58 3022G 20.8 12
2982 6.41 19 3023 263 9
2982G 16.3 9 3023G 103 5
2985 64.4 9 3024 58.8 7
2985G 2.44 8 3024G 7.09 10
2987 21.0 11 3025 35.2 6
2987G 37.6 4 3025G 42.5 8
2996 10.8 9 3027 7.15 6
2996G 24.0 2 3027G 4.24 18
2997 7.75 19 3028 6.89 37
2997G 151 1 3028G 7.23 22
3004 46.5 14 3030 46.2 7
3004G 1.93 91 3030G 128 3
3005 2.35 108 3032 53.2 9
3005G 6.96 27 3032G 13.0 1
3010 4.13 26 3033 4.61 17
3010G 2.10 49 3033G 12.0 5
3011 59.1 5 3036 284 12
3011G 41.7 5 3036G 18.2 10
3012 9.71 20 3041 6.90 12
3012G 89.9 2 3041G 22.9 2
3013 20.2 20 3042 9.46 34
3013G 13.2 4 3042G 85.5 3
3014 213 4 3043 9.26 29
3014G 36.8 3 3043G 13.1 22
TABLE 12
V 3-20J 1
Common Light Chain Antibodies
100 nM Antigen E 100 nM Antigen E
Antibody Antibody
K (nM) T (min) K (nM) T (min)
D 1/2 D 1/2
2968 5.50 8 2973 5.35 39
2968G 305 0 2973G 11.0 44
2969 34.9 2 2974 256 0
2969G 181 1 2974G 138 0
2970G 12.3 3 2975 38.0 2
2971G 32.8 22 2975G 134 1
2972 6.02 13 2976 6.73 10
2972G 74.6 26 2976G 656 8
The binding affinities of common light chain antibodies comprising the
rearrangements shown in Tables 5 and 6 vary, with nearly all exhibiting a K in the
nanomolar range. The affinity data is consistent with the common light chain antibodies
resulting from the combinatorial association of rearranged variable domains described in
Tables 5 and 6 being high-affinity, clonally selected, and somatically mutated. Coupled with
data previously shown, the common light chain antibodies described in Tables 5 and 6
comprise a collection of diverse, high-affinity antibodies that exhibit specificity for one or
more epitopes on Antigen E.
Example 10. Determination of Binding Specificities of Antigen-Specific Common Light
Chain Antibodies by LUMINEX™ Assay
Selected anti-Antigen E common light chain antibodies were tested for their
ability to bind to the ECD of Antigen E and Antigen E ECD variants, including the
cynomolgous monkey ortholog (Mf Antigen E), which differs from the human protein in
approximately 10% of its amino acid residues; a deletion mutant of Antigen E lacking the last
amino acids from the C-terminal end of the ECD (Antigen E- CT); and two mutants
containing an alanine substitution at suspected locations of interaction with Ligand Y
(Antigen E-Ala1 and AntigenE-Ala2). The Antigen E proteins were produced in CHO cells
and each contained a myc-myc-His C-terminal tag.
For the binding studies, Antigen E ECD protein or variant protein (described
above) from 1 mL of culture medium was captured by incubation for 2 hr at room
temperature with 1 x 10 microsphere (LUMINEX™) beads covalently coated with an anti-
myc monoclonal antibody (MAb 9E10, hybridoma cell line CRL-1729™; ATCC, Manassas,
VA). The beads were then washed with PBS before use. Supernatants containing anti-
Antigen E common light chain antibodies were diluted 1:4 in buffer and added to 96-well filter
plates. A mock supernatant with no antibody was used as negative control. The beads
containing the captured Antigen E proteins were then added to the antibody samples (3000
beads per well) and incubated overnight at 4°C. The following day, the sample beads were
washed and the bound common light chain antibody was detected with a R-phycoerythrin-
conjugated anti-human IgG antibody. The fluorescence intensity of the beads
(approximately 100 beads counted for each antibody sample binding to each Antigen E
protein) was measured with a LUMINEX™ flow cytometry-based analyzer, and the median
fluorescence intensity (MFI) for at least 100 counted beads per bead/antibody interaction
was recorded. Results are shown in Tables 13 and 14.
TABLE 13
V 1-39J 5 Common Light Chain Antibodies
Mean Fluorescence Intensity (MFI)
Antibody
Antigen E- Antigen E- Antigen E- Antigen E-
Mf Antigen E
ECD CT Ala1 Ala2
2948 1503 2746 4953 3579 1648
2948G 537 662 2581 2150 863
2949 3706 4345 8169 5678 5142
2949G 3403 3318 7918 5826 5514
2950 3296 4292 7756 5171 4749
2950G 2521 2408 7532 5079 3455
2952 3384 1619 1269 168 911
2952G 3358 1001 108 55 244
2954 2808 3815 7114 5039 3396
2954G 2643 2711 7620 5406 3499
2955 1310 2472 4738 3765 1637
2955G 1324 1802 4910 3755 1623
2964 5108 1125 4185 346 44
2964G 4999 729 4646 534 91
2978 6986 2800 14542 10674 8049
2978G 5464 3295 11652 8026 6452
2982 4955 2388 13200 9490 6772
2982G 3222 2013 8672 6509 4949
2985 1358 832 4986 3892 1669
2985G 43 43 128 244 116
2987 3117 1674 7646 5944 2546
2987G 3068 1537 9202 6004 4744
2996 4666 1917 12875 9046 6459
2996G 2752 1736 8742 6150 4873
2997 5164 2159 12167 8361 5922
2997G 658 356 3392 2325 1020
3004 2794 1397 8542 6268 3083
3004G 2753 1508 8267 5808 4345
3005 5683 2221 12900 9864 5868
3005G 4344 2732 10669 7125 5880
3010 4829 1617 2642 3887 44
3010G 3685 1097 2540 3022 51
3011 2859 2015 7855 5513 3863
3011G 2005 1072 6194 4041 3181
3012 3233 2221 8543 5637 3307
3012G 968 378 3115 2261 1198
3013 2343 1791 6715 4810 2528
3013G 327 144 1333 1225 370
3014 1225 1089 5436 3621 1718
3014G 1585 851 5178 3705 2411
3015 3202 2068 8262 5554 3796
3015G 1243 531 4246 2643 1611
3016 4220 2543 8920 5999 5666
3016G 2519 1277 6344 4288 4091
3017 3545 2553 8700 5547 5098
3017G 1972 1081 5763 3825 3038
3018 2339 1971 6140 4515 2293
3018G 254 118 978 1020 345
3019 5235 1882 7108 4249 54
3019G 4090 1270 4769 3474 214
3020 3883 3107 8591 6602 4420
3020G 2165 1209 6489 4295 2912
3021 1961 1472 6872 4641 2742
3021G 2091 1005 6430 3988 2935
3022 2418 793 7523 2679 36
3022G 2189 831 6182 3051 132
3023 1692 1411 5788 3898 2054
3023G 1770 825 5702 3677 2648
3024 1819 1467 6179 4557 2450
3024G 100 87 268 433 131
3025 1853 1233 6413 4337 2581
3025G 1782 791 5773 3871 2717
3027 4131 1018 582 2510 22
3027G 3492 814 1933 2596 42
3028 4361 2545 9884 5639 975
3028G 2835 1398 7124 3885 597
3030 463 277 1266 1130 391
3030G 943 302 3420 2570 1186
3032 2083 1496 6594 4402 2405
3032G 295 106 814 902 292
3033 4409 2774 8971 6331 5825
3033G 2499 1234 6745 4174 4210
3036 1755 1362 6137 4041 1987
3036G 2313 1073 6387 4243 3173
3041 3674 2655 8629 5837 4082
3041G 2519 1265 6468 4274 3320
3042 2653 2137 7277 5124 3325
3042G 1117 463 4205 2762 1519
3043 3036 2128 7607 5532 3366
3043G 2293 1319 6573 4403 3228
TABLE 14
V 3-20J 1 Common Light Chain Antibodies
Mean Fluorescence Intensity (MFI)
Antibody
Antigen E- Antigen E- Antigen E- Antigen E-
Mf Antigen E
ECD CT Ala1 Ala2
2968 6559 3454 14662 3388 29
2968G 2149 375 9109 129 22
2969 2014 1857 7509 5671 3021
2969G 1347 610 6133 4942 2513
2970 5518 1324 14214 607 32
2970G 4683 599 12321 506 31
2971 501 490 2506 2017 754
2971G 578 265 2457 2062 724
2972 2164 2158 8408 6409 3166
2972G 1730 992 6364 4602 2146
2973 3527 1148 3967 44 84
2973G 1294 276 1603 28 44
2974 1766 722 8821 241 19
2974G 2036 228 8172 135 26
2975 1990 1476 8669 6134 2468
2975G 890 315 4194 3987 1376
2976 147 140 996 1079 181
2976G 1365 460 6024 3929 1625
The anti-Antigen E common light chain antibody supernatants exhibited high
specific binding to the beads linked to Antigen E-ECD. For these beads, the negative control
mock supernatant resulted in negligible signal (<10 MFI) when combined with the Antigen E-
ECD bead sample, whereas the supernatants containing anti-Antigen E common light chain
antibodies exhibited strong binding signal (average MFI of 2627 for 98 antibody
supernatants; MFI > 500 for 91/98 antibody samples).
As a measure of the ability of the selected anti-Antigen E common light chain
antibodies to identify different epitopes on the ECD of Antigen E, the relative binding of the
antibodies to the variants were determined. All four Antigen E variants were captured to the
anti-myc LUMINEX™ beads as described above for the native Antigen E-ECD binding
studies, and the relative binding ratios (MFI /MFI ) were determined. For 98
variant Antigen E-ECD
tested common light chain antibody supernatants shown in Tables 12 and 13, the average
ratios (MFI /MFI ) differed for each variant, likely reflecting different capture
variant Antigen E-ECD
amounts of proteins on the beads (average ratios of 0.61, 2.9, 2.0, and 1.0 for Antigen E-
CT, Antigen E-Ala1, Antigen E-Ala2, and Mf Antigen E, respectively). For each protein
variant, the binding for a subset of the 98 tested common light chain antibodies showed
greatly reduced binding, indicating sensitivity to the mutation that characterized a given
variant. For example, 19 of the common light chain antibody samples bound to the Mf
Antigen E with MFI /MFI of <8%. Since many in this group include high or
variant Antigen E-ECD
moderately high affinity antibodies (5 with K < 5nM, 15 with K < 50 nM), it is likely that the
lower signal for this group results from sensitivity to the sequence (epitope) differences
between native Antigen E-ECD and a given variant rather than from lower affinities.
These data establish that the common light chain antibodies described in Tables
and 6 represent a diverse group of Antigen-E-specific common light chain antibodies that
specifically recognize more than one epitope on Antigen E.
Example 11. Light Chain Shuffling in Common Light Chain Antibodies
Heavy chains of selected antigen-specific common light chain antibodies were
tested for binding to Antigen E after repairing the heavy chains with either a germline V 1-
39J 5 or a germline V 3-20J 1 engineered light chain (as described in Example 1).
Briefly, 247 heavy chains of Antigen E-specific common light chain antibodies
(V 1-39J 5 and V 3-20J 1) were transfected with either a germline V 1-39 or a germline
V 3-20 engineered light chain and rescreened for binding to Antigen E by a LUMINEX™
assay (as described in Example 7 and Example 10). Binding to Antigen E was confirmed by
BIACORE™ (as described in Example 9). The results are shown in Table 15.
As shown in this Example, twenty-eight common light chain antibodies specific
for Antigen E were capable of binding to Antigen E when repaired with a germline form of the
light chain.
TABLE 15
Original Light Chain Repaired Light Chain No. Tested No. Confirmed Binders
1-39 1-39 198 23
3-20 3-20 49 5
Example 12. Heavy Chain Gene Usage and Somatic Hypermutation Frequency in
Common Light Chain Antibodies
Heavy and light chain sequences (>6000) of antibodies raised in
VELCOIMMUNE® mice (e.g., US 6,596,541 and US 7,105,348) were compiled with heavy
and light chain sequences (>600) of common light chain antibodies obtained by a multi-
antigen immunization scheme employing the engineered light chain mice (described above)
to compare heavy chain gene segment usage and somatic hypermutation frequencies of the
antibody chains.
Heavy Chain Gene Usage. Heavy and light chain sequences obtained from
VELOCIMMUNE® mice containing a replacement of the endogenous mouse heavy chain
locus with human V , D , and J gene segments and a replacement of the endogenous
H H H
mouse light chain locus with either the engineered germline V 1-39J 5 human light chain
region or the engineered germline V 3-20J 1 human light chain region (as described in
Example 2) immunized with a human cell-surface receptor (Antigen E), a heterodimer of two
human cell-surface glycoproteins (Antigen F), a human cytokine receptor (Antigen G) and a
human tumor differentiation antigen (Antigen H) were analyzed for heavy chain gene
segment usage and V and J gene segments were recorded. Results are shown in Tables
16 – 18. Percentages in Tables 16 – 18 represent rounded values and in some cases may
not equal 100% when added together.
Table 16 sets forth the percent heavy chain family usage for antibodies from
VELCOIMMUNE® mice (VI), antibodies from VELCOIMMUNE® mice having a cognate V 1-
39 light chain (VI – V 1-39), antibodies from V 1-39 engineered light chain mice (V 1-39),
antibodies from VELCOIMMUNE® mice having a cognate V 3-20 light chain (VI – V 3-20),
and antibodies from V 3-20 engineered light chain mice (V 3-20). Table 17 sets forth the
percent V and J gene usage for antibodies from VELCOIMMUNE® mice (VI), antibodies
from VELCOIMMUNE® mice having a cognate V 1-39 light chain (VI – V 1-39), antibodies
from V 1-39 engineered light chain mice (V 1-39), antibodies from VELCOIMMUNE® mice
having a cognate V 3-20 light chain (VI – V 3-20), and antibodies from V 3-20 engineered
light chain mice (V 3-20). Table 18 sets forth the percent V gene usage for antibodies from
V 1-39 engineered light chain mice (V 1-39 Mice) from each immunization group (Antigens
E, F, G and H) and the percent V gene usage for antibodies from V 3-20 engineered light
chain mice (V 3-20 Mice) from selected immunization groups (Antigens E and G).
As shown in this Example, heavy chain gene usage for antigens tested in V 1-
39J 5-engineered light chain mice was characterized by a preponderance of V family III
subgroups (V 3-7, V 3-9, V 3-11, V 3-13, V 3-20, V 3-23, V 3-30, V 3-33 and V 3-48).
H H H H H H H H H
Notable usage of other V family subgroups was characterized by usage of V 1-18, V 1-69,
H H H
V 2-5, V 4-59 and V 6-1. For antigens tested in V 3-20J 1 engineered light chain mice,
H H H
heavy chain gene usage was characterized by a preponderance of V family III, V family IV
and V family V subgroups (V 3-11, V 3-30, V 3-33, V 4-39, V 4-59 and V 5-51). Notable
H H H H H H H
usage of other V family subgroups was characterized by usage of V 1-18, V 1-69, V 2-70
H H H H
and V 6-1.
Somatic Hypermutation Frequency. Heavy and light chains from antibodies
raised in VELCOIMMUNE® mice and the engineered light chain mice (described above)
were aligned to germline sequences according to the heavy and light chain gene usage
demonstrated for each heavy and/or light chain. Amino acid changes for each framework
region (FW) and complementarity determining region (CDR) for both heavy and light chain of
each sequence were calculated. Results are shown in Tables 19 – 22. Percentages in
Tables 21 – 24 represent rounded values and in some cases may not equal 100% when
added together.
Table 19 sets forth the number of amino acid (AA) changes observed in each FW
and CDR region of heavy chains of antibodies from VELCOIMMUNE® mice, heavy chains of
antibodies from V 1-39 engineered light chain mice (V 1-39 Mice) and heavy chains of
antibodies from V 3-20 engineered light chain mice (V 3-20 Mice). Table 20 sets forth the
number of amino acid (AA) changes observed in each FW and CDR region of light chains of
antibodies from VELCOIMMUNE® mice, the light chain of antibodies from V 1-39
engineered mice (V 1-39 Mice) and the light chain of antibodies from V 3-20 engineered
mice (V 3-20 Mice). Table 21 sets forth the number of amino acid (AA) changes observed
in each FW and CDR region of heavy chains of antibodies from V 1-39 engineered light
chain mice (V 1-39 Mice) for selected immunization groups (Antigens E, F and H). Table 22
sets forth the number of amino acid (AA) changes observed in each FW and CDR region of
heavy chains of antibodies from V 3-20 engineered light chain mice (V 3-20 Mice) for
selected immunization groups (Antigens E and G).
TABLE 16
V Family VI VI – V 1-39 V 1-39 VI – V 3-20 V 3-20
1 9.0 14.8 3.3 7.1 4.9
2 2.2 1.8 4.6 0 1.6
3 77.8 69.8 77.3 61.4 29.5
4 8.4 8.3 11.2 27.1 39.3
0.9 0 0.7 4.3 23.0
6 1.7 5.3 3.0 0 1.6
TABLE 17
V Gene VI VI – V 1-39 V 1-39 VI – V 3-20 V 3-20
1-2 3.9 8.3 0 2.9 0
1-3 0 0 0 0 0
1-8 1.3 0.6 0 1.4 0
1-18 3.0 0.6 1.3 2.1 1.6
1-24 0.4 3.6 0 0.7 0
1-46 0.1 0 0 0 0
1-58 0 0 0 0 0
1-69 0.3 1.8 2.0 0 3.3
2-5 1.9 0 4.6 0 0
2-26 0.2 1.8 0.0 0 0
2-70 0.1 0 0 0 1.6
3-7 3.0 14.8 0 1.4 0
3-9 8.5 3.6 29.6 16.4 0
3-11 5.4 10.7 0 7.1 1.6
3-13 3.2 1.8 0.7 2.1 0
3-15 4.0 4.7 0.3 0.7 0
3-20 1.0 0.6 0.3 5.0 0
3-21 0.8 0.6 0 2.1 0
3-23 20.4 8.9 3.3 8.6 0
3-30 17.6 4.1 35.2 12.9 1.6
3-33 12.6 14.8 0 5.0 26.2
3-43 0.2 0.6 0 0 0
3-48 0.8 1.2 7.2 0 0
3-53 0.3 3.6 0.3 0 0
3-64 0 0 0.3 0 0
3-72 0 0 0 0 0
3-73 0 0 0 0 0
4-31 2.7 0 0.7 8.6 0
4-34 1.8 0.6 0.3 14.3 0
4-39 1.6 0.6 3.0 2.1 14.8
4-59 2.3 7.1 7.2 2.1 24.6
-51 0.9 0 0.7 4.3 23.0
6-1 1.7 5.3 3.0 0 1.6
J Gene VI VI – V 1-39 V 1-39 VI – V 3-20 V 3-20
1 1.5 1.2 7.1 0 0
2 4.5 2.4 0.7 5.0 26.9
3 10.5 16.6 13.1 13.6 26.9
4 44.0 34.3 32.3 50.7 9.6
9.6 10.1 16.8 7.9 1.9
6 29.7 35.5 30.0 22.9 34.6
TABLE 18
V 1-39 Mice V 3-20 Mice
V Gene
Antigen E Antigen F Antigen G Antigen H Antigen E Antigen G
1-2 0 0 0 0 0 0
0 0 0 0 0 0
1-8 0 0 0 0 0 0
1-18 0 0 0 8.3 0 3.1
1-24 0 0 0 0 0 0
1-46 0 0 0 0 0 0
1-58 0 0 0 0 0 0
1-69 2.9 0 25.0 0 0 6.3
2-5 8.2 0 0 0 0 0
2-26 0 0 0 0 0 0
2-70 0 0 0 0 0 3.1
3-7 0 0 0 0 0 0
3-9 1.2 98.8 0 14.6 0 0
3-11 0 0 0 0 0 3.1
0 0 0 0
3-13 0.6 25.0
3-15 0 1.2 0 0 0 0
3-20 0 0 25.0 0 0 0
3-21 0 0 0 0 0 0
3-23 4.1 0 25.0 4.2 0 0
3-30 62.9 0 0 0 3.4 0
3-33 0 0 0 0 13.8 37.5
3-43 0 0 0 0 0 0
3-48 0.6 0 0 43.8 0 0
3-53 1.6 0 0 0 0 0
3-64 1.6 0 0 0 0 0
3-72 0 0 0 0 0 0
3-73 0 0 0 0 0 0
4-31 0 0 0 4.2 0 0
0 0 0 0 0
4-34 2.1
4-39 5.3 0 0 0 31.0 0
4-59 11.8 0 0 4.2 3.4 43.8
-51 1.2 0 0 0 48.3 0
6-1 0 0 0 18.8 0 3.1
TABLE 19
Heavy Chains of Antibodies from VELCOIMMUNE® Mice
# AA Changes
FW1 CDR1 FW2 CDR2 FW3 CDR3
0 63 32 36 26 12 82
1 23 32 41 31 22 17
2 9 25 17 23 27 1
3 4 10 5 16 13 0
4 0 1 1 3 12 0
>5 1 0 0 1 14 0
Heavy Chains of Antibodies from V 1-39 Mice
# AA Changes
FW1 CDR1 FW2 CDR2 FW3 CDR3
0 65 8 34 30 9 37
1 25 26 35 34 19 54
2 9 44 23 20 33 9
3 1 19 8 12 22 0
4 0 3 0 5 11 0
>5 1 0 0 0 7 0
Heavy Chains of Antibodies from V 3-20 Mice
# AA Changes
FW1 CDR1 FW2 CDR2 FW3 CDR3
0 57 8 54 16 8 93
1 41 43 34 39 21 7
2 2 25 10 18 20 0
3 0 15 2 21 13 0
4 0 10 0 3 20 0
>5 0 0 0 2 18 0
TABLE 20
Light Chains of Antibodies from VELCOIMMUNE® Mice
# AA Changes
FW1 CDR1 FW2 CDR2 FW3 CDR3
0 65 24 49 60 33 23
1 24 20 34 31 27 38
2 9 27 16 9 18 28
3 1 20 1 0 14 7
4 0 7 0 0 4 3
>5 1 1 0 0 3 0
Light Chains of Antibodies from V 1-39 Mice
# AA Changes
FW1 CDR1 FW2 CDR2 FW3 CDR3
0 91 75 80 90 71 63
1 9 19 17 10 21 27
2 0 5 1 1 5 8
3 0 0 1 0 2 1
4 0 0 0 0 2 1
>5 0 0 0 0 0 0
Light Chains of Antibodies from V 3-20 Mice
# AA Changes
FW1 CDR1 FW2 CDR2 FW3 CDR3
0 90 47 93 97 63 57
1 10 27 3 3 20 43
2 0 27 3 0 17 0
3 0 0 0 0 0 0
4 0 0 0 0 0 0
>5 0 0 0 0 0 0
TABLE 21
Heavy Chains of Anti-Antigen E Antibodies from V 1-39 Mice
# AA Changes
FW1 CDR1 FW2 CDR2 FW3 CDR3
0 75 8 49 41 14 36
1 21 25 33 35 25 52
2 4 43 14 18 28 12
3 0 20 4 5 16 0
4 0 5 0 1 12 0
>5 1 0 0 0 5 0
Heavy Chains of Anti-Antigen F Antibodies from V 1-39 Mice
# AA Changes
FW1 CDR1 FW2 CDR2 FW3 CDR3
0 52 0 6 6 2 15
1 35 24 32 35 15 78
2 11 59 46 22 49 7
3 0 17 16 24 29 0
4 0 0 0 12 4 0
>5 1 0 0 0 1 0
Heavy Chains of Anti-Antigen H Antibodies from V 1-39 Mice
# AA Changes
FW1 CDR1 FW2 CDR2 FW3 CDR3
0 54 21 29 33 4 77
1 17 35 50 27 6 23
2 23 21 15 21 25 0
3 6 21 4 15 27 0
4 0 2 2 2 15 0
>5 0 0 0 2 23 0
TABLE 22
Heavy Chains of Anti-Antigen E Antibodies from V 3-20 Mice
# AA Changes
FW1 CDR1 FW2 CDR2 FW3 CDR3
0 79 17 62 24 17 90
1 21 28 34 55 31 10
2 0 28 3 21 24 0
3 0 14 0 0 10 0
4 0 14 0 0 3 0
>5 0 0 0 0 14 0
Heavy Chains of Anti-Antigen G Antibodies from V 3-20 Mice
# AA Changes
FW1 CDR1 FW2 CDR2 FW3 CDR3
0 38 0 47 9 0 97
1 59 56 34 25 13 3
2 3 22 16 16 16 0
3 0 16 3 41 16 0
4 0 6 0 6 34 0
>5 0 0 0 3 22 0
Example 13. Binding Affinity of Bispecific Antibodies Having Universal Light Chains
Fully human bispecific antibodies were constructed from cloned human heavy
chain variable regions of selected monospecific anti-Antigen E common light chain
antibodies (described in Example 5) using standard recombinant DNA techniques known in
the art. Table 23 sets forth the pairing of human heavy chains (HC-1 and HC-2) from
selected parental monospecific antibodies; each pair employed with a germline rearranged
human V 1-39/J 1 light chain for construction of each bispecific antibody.
Binding of bispecific or parental monospecific anti-Antigen E antibodies to the
extracellular domain (ECD) of Antigen E was determined using a real-time surface plasmon
resonance biosensor assay on a BIACORE™ 2000 instrument (GE Healthcare). A CM5
BIACORE™ sensor surface derivatized with anti-c-myc-specific monoclonal antibody
(Clone# 9E10) using EDC-NHS chemistry was used to capture the C-terminal myc-myc-
hexahistidine tagged ECD of Antigen E (AntigenE-mmh). Around 190 RUs of AntigenE-
mmh was captured on the BIACORE™ sensor surface, followed by the injection of 300nM
and 50nM concentrations of different bispecific or parental monospecific anti-Antigen E
antibodies at a flow rate of 50 µl/min. The experiment was performed at 25ºC in HBST
running buffer (0.01M HEPES pH 7.4, 0.15M NaCl, 3mM EDTA, 0.05% v/v Surfactant P20).
The amount of antibody binding to AntigenE-mmh surface at 300nM concentration was
recorded three seconds before the end of antibody injection and plotted.
Table 24 and set forth the binding responses (BIACORE™ units; RU)
observed for each bispecific antibody (BsAb) and monospecific parental antibody (PAb-1,
PAb-2). Since each antibody was injected under saturating conditions over an identical
AntigenE-mmh surface, the binding response reflects the binding stoichiometry for each
antibody binding to the antigen capture surface.
As shown in this Example, the observed binding response for each bispecific
antibody was approximately 2-fold greater than the binding response for each parental
monospecific antibody (Table 24 and , demonstrating functional construction of
bispecific antibodies using heavy chains of antigen-specific monoclonal antibodies and a
common light chain where each Fab arm in the bispecific antibody molecule binds
simultaneously to distinct epitopes on the extracelluar domain of a cell surface receptor
(Antigen E; see , bottom left).
TABLE 23
Bispecific Antibody Parent HC-1 Parent HC-2
3108 2952 2978
3109 2978 3022
3111 2952 3005
3112 3022 3005
TABLE 24
Binding Response (RU)
Bispecific Antibody
PAb-1 PAb-2 BsAb
3108 236 229 485
3109 236 197 408
3111 202 229 435
3112 202 197 345
Example 14. Generation and Analysis of Mice Expressing Two Human Light Chains
Using the methods described above in Example 2, two additional engineered light
chain loci containing two human V gene segments (e.g., a human V 1-39 and human V 3-
gene segment) were constructed (. One engineered light chain locus contained
two human V gene segments and five human J gene segments in unrearranged
configuration (DLC-5J). The second engineered light chain locus contained two human V
gene segments and one human J gene segment in unrearranged configuration (DLC-1J).
For each of the two additional engineered light chain loci, the human gene segments were
flanked 3’ with recombination signal sequences to allow for in vivo rearrangement of the
human gene segments in B cells.
Modified BAC DNA clones separately containing each of the the engineered light
chain loci operably linked to mouse sequences (i.e., upstream and downstream sequences
of the endogenous immunoglobulin light chain locus) were confirmed by PCR using
primers located at sequences within each engineered light chain locus containing the two
human V gene segments followed by electroporation into ES cells to create mice that
express either of the two human V gene segments (as described above). Positive ES cell
clones that contain either of the engineered light chain loci described above were confirmed
by TAQMAN™ screening and karyotyping using probes specific for the engineered light
chain loci (as described above). Confirmed ES cell clones were then used to implant female
mice to give rise to a litter of pups expressing a human light chain variable domain fused
with a mouse C domain, referred to herein as Dual Light Chain (DLC) mice.
Alternatively, ES cells bearing the engineered light chain locus may be
transfected with a construct that expresses FLP in order to remove the FRTed neomycin
cassette introduced by the targeting construct. Optionally, the neomycin cassette is
removed by breeding to mice that express FLP recombinase (e.g., US 6,774,279).
Optionally, the neomycin cassette is retained in the mice.
Flow Cytometry. B cell populations and B cell development in DLC mice were
validated by flow cytometry analysis of splenocyte and bone marrow preparations. Cell
suspensions from mice homozygous for two human V gene segments and five human J
gene segments (n=4), mice homozygous for two human V gene segments and one human
J gene segment (n=4), and wild type mice (n=4) were made using standard methods
(described above) and stained with fluorescently labeled antibodies (as described in
Example 3).
Briefly, 1x10 cells were incubated with anti-mouse CD16/CD32 (clone 2.4G2, BD
Pharmigen) on ice for 10 minutes, followed by labeling with the following antibody cocktail for
minutes on ice: APC-H7 conjugated anti-mouse CD19 (clone 1D3, BD Pharmigen),
Pacific Blue conjugated anti-mouse CD3 (clone 17A2, BioLegend), FITC conjugated anti-
mouse Ig (clone 187.1, BD Pharmigen) or anti-mouse CD43 (clone 1B11, BioLegend), PE
conjugated anti-mouse Ig (clone RML-42, BioLegend) or anti-mouse c-kit (clone 2B8,
BioLegend), PerCP-Cy5.5 conjugated anti-mouse IgD (BioLegend), PE-Cy7 conjugated anti-
mouse IgM (clone II/41, eBioscience), APC conjugated anti-mouse B220 (clone RA3-6B2,
eBioscience). Following staining, cells were washed and fixed in 2% formaldehyde. Data
acquisition was performed on an LSRII flow cytometer and analyzed with FlowJo (Tree Star,
+ - + + - + - + -
Inc.). Gating: total B cells (CD19 CD3 ), Ig B cells (Ig Ig CD19 CD3 ), Ig B cells (Ig
+ + -
Ig CD19 CD3 ). Results for the bone marrow compartment are shown in A – B. Results for the splenic compartment are shown in A – .
As shown in this Example, DLC-5J mice demonstrate normal B cell populations
within the splenic and bone marrow compartments (A – 16). DLC-5J mice
demonstrated immature, mature and pre/pro B cell populations within the bone marrow
compartment that are substantially the same as observed in wild-type litter mates. In fact,
the DLC-5J locus was capable of competing with the endogenous light chain locus to yield
a : ratio that is substantially the same as that observed in wild-type mice (B). Also,
DLC-5J mice demonstrate a normal peripheral B cell development as progression of B cells
through various stages in the splenic compartment (e.g., immature, mature, T1, T2 T3,
marginal zone precursor, marginal zone, follicular-I, follicular-II, etc.) occurs in a manner
substantially the same as observed in wild type mice (A – 16). In contrast, DLC-1J
mice demonstrated a lower overall number of B cells and an increased light chain usage
as compared to the engineered light chain (data not shown).
Dual Light Chain Expression. Expression of both human V gene segments
was analyzed in homozygous mice using a quantitative PCR assay in accordance with in
Example 3. Briefly, CD19 B cells were purified from bone marrow and whole spleens of
wild type mice, mice homozygous for a replacement of the mouse heavy chain and light
chain variable loci with corresponding human heavy chain and light chain variable region
loci (H ), as well as mice homozygous for an engineered light chain loci containing two
human V gene segments and either five human J gene segments (DLC-5J) or one human
J gene segment (DLC-1J). Relative expression was normalized to expression of mouse C
region (n=3 to 5 mice per group). Results are shown in and .
Expression of light chains containing a rearranged human V 3-20 or human V 1-
39 gene segment were detected in both the bone marrow and spleen of DLC-5J and DLC-1J
mice ( and ). In the bone marrow compartment, expression of both human
V 3derived and human V 1derived light chains in both strains of DLC mice was
significantly higher as compared to mice comprising a replacement of mouse V and J
gene segment with corresponding human V and J gene segments (H ; ). Human
V 3derived light chain expression was observed at about six-fold (DLC-5J) to fifteen-fold
(DLC-1J) higher than in H mice. DLC-1J mice demonstrated about two-fold higher
expression of human V 3derived light chains over DLC-5J mice in the bone marrow
compartment. Human V 1derived light chain expression was observed at about six-fold
(DLC-5J) to thirteen-fold (DLC-1J) higher than in H mice. DLC-1J mice demonstrated
about two-fold higher expression of human V 1derived light chains over DLC-5J mice in
the bone marrow compartment.
In the splenic compartment, expression of both human V 3derived and
human V 1derived light chains in both strains of DLC mice was significantly higher as
compared to H mice (). Human V 3derived light chain expression was
observed at about four-fold (DLC-5J) and eight-fold (DLC-1J) higher than in H mice. DLC-
1J mice demonstrated about two-fold higher expression of human V 3derived light
chains over DLC-5J mice in the splenic compartment. Human V 1derived light chain
expression was observed at about four-fold (DLC-5J) to five-fold (DLC-1J) higher than in H
mice. DLC-1J mice demonstrated similar expression of human V 1derived light chains
as compared to DLC-5J mice in the splenic compartment.
Human V /J Usage in DLC-5J Mice. Mice homozygous for two unrearranged
human V gene segments and five unrearranged human J gene segments (DLC-5J) were
analyzed for human V /J gene segment usage in splenic B cells by reverse-transcriptase
polymerase chain reaction (RT-PCR).
Briefly, spleens from homozygous DLC-5J (n=3) and wild type (n=2) mice were
harvested and meshed in 10 mL of RPMI 1640 (Sigma) containing 10% heat-inactivated
fetal bovine serum using frosted glass slides to create single cell suspensions. Splenocytes
were pelleted with a centrifuge (1200 rpm for five minutes) and red blood cells were lysed in
mL of ACK lysing buffer (GIBCO) for three minutes. Splenocytes were diluted with PBS
(Irvine Scientific), filtered with a 0.7 μm cell strainer and centrifuged again to pellet cells,
which was followed by resuspension in 1 mL of PBS.
RNA was isolated from pelleted splenocytes using AllPrep DNA/RNA mini kit
(Qiagen) according to manufacturer’s specifications. RT-PCR was performed on splenocyte
RNA using 5’ RACE (Rapid Amplification of cDNA ends) System with primers specific for the
mouse C gene according to manufacturer’s specifications (Invitrogen). The primers
specific for the mouse C gene were 3’ mIg C RACE1 (AAGAAGCACA CGACTGAGGC
AC; SEQ ID NO: 34) and mIg C3’-1 (CTCACTGGAT GGTGGGAAGA TGGA; SEQ ID NO:
). PCR products were gel-purified and cloned into pCR®2.1-TOPO® vector (TOPO® TA
Cloning® Kit, Invitrogen) and sequenced with M13 Forward (GTAAAACGAC GGCCAG;
SEQ ID NO: 36) and M13 Reverse (CAGGAAACAG CTATGAC; SEQ ID NO: 37) primers
located within the vector at locations flanking the cloning site. Ten clones from each spleen
sample were sequenced. Sequences were compared to the mouse and human
immunoglobulin sets from the IMGT/V-QUEST reference directory sets to determine V /J
usage. Table 25 sets forth the V /J combinations for selected clones observed in RT-PCR
clones from each splenocyte sample. Table 26 sets forth the amino acid sequence of the
human V /human J and human J /mouse C junctions of selected RT-PCR clones from
DLC-5J homozygous mice. Lower case letters indicate mutations in the amino acid
sequence of the variable region or non-template additions resulting from N and/or P
additions during recombination.
As shown in this Example, mice homozygous for two unrearranged human V
gene segments and five unrearranged human J gene segments (DLC-5J) operably linked
to the mouse C gene are able to productively recombine both human V gene segments to
multiple human J gene segments to produce a limited immunoglobulin light chain
repertoire. Among the rearrangements in DLC-5J homozygous mice shown in Table 25,
unique human V /J rearrangements were observed for V 1-39/J 2 (1), V 1-39/J 3 (1),
V 3-20/J 1 (7), V 3-20/J 2 (4) and V 3-20/J 3 (1). Further, such unique rearrangements
demonstrated junctional diversity through the presence of unique amino acids within the
CDR3 region of the light chain (Table 26) resulting from either mutation and/or the
recombination of the human V and J gene segments during development. All the
rearrangements showed functional read through into mouse C (Table 26).
Taken together, these data demonstrate that mice engineered to present a
choice of no more than two human V gene segments, both of which are capable of
rearranging (e.g., with one or more and, in some embodiments, up to five human J gene
segments) and encoding a human V domain of an immunoglobulin light chain have B cell
numbers and development that is nearly wild-type in all aspects. Such mice produce a
collection of antibodies having immunoglobulin light chains that have one of two possible
human V gene segments present in the collection. This collection of antibodies is produced
by the mouse in response to antigen challenge and are associated with a diversity of reverse
chimeric (human variable/mouse constant) heavy chains.
TABLE 25
Mouse ID No. Genotype Clone V /J Combination
1-2 1-39/3
1-4 3-20/2
1089451 DLC-5J
1-7 3-20/1
1-8 3-20/2
2-2 3-20/1
2-3 3-20/1
1089452 DLC-5J 2-6 3-20/2
2-8 3-20/2
2-9 3-20/1
2-10 1-39/2
3-1 3-20/1
3-2 3-20/1
1092594 DLC-5J 3-4 3-20/1
3-6 3-20/3
3-9 3-20/2
1-1 19-93/1
1-2 6-25/1
1-3 4-91/5
1092587 WT 1-5 3-10/4
1-6 4-86/4
1-8 19-93/1
1-10 19-93/2
2-1 19-93/1
2-3 6-20/5
2-4 6-25/5
2-5 1-117/1
1092591 WT
2-6 8-30/1
2-7 8-19/2
2-8 8-30/1
2-10 1-117/1
TABLE 26
Sequence of hV /hJ /mC Junction
Clone V /J SEQ ID NO:
(CDR3 underlined, mIg C italics)
2-10 1-39/2 QPEDFATYYCQQSYSTPYTFGQGTKLEIKRADAAPTVSI 38
1-2 1-39/3 QPEDFATYYCQQSYSTPFTFGPGTKVDIKRADAAPTVSI 39
1-7 3-20/1 EPEDFAVYYCQQYGSSPrTFGQGTKVEIKRADAAPTVSI 40
2-2 3-20/1 EPEDFAVYYCQQYGSSrTFGQGTKVEIKRADAAPTVSI 41
2-3 3-20/1 EPEDFAVYYCQQYGSSPWTFGQGTKVEIKRADAAPTVSI 42
2-9 3-20/1 dPEDFAVYYCQQYGSSPrTFGQGTKVEIKRADAAPTVSI 44
3-1 3-20/1 EPEDFAVYYCQQYGSSPrTFGQGTKVEIKRADAAPTVSI 45
3-2 3-20/1 EPEDFAVYYCQQYGSSPWTFGQGTKVEIKRADAAPTVSI 46
3-4 3-20/1 EPEDFAVYYCQQYGSSPPTFGQGTKVEIKRADAAPTVSI 47
3-9 3-20/2 EPEDFAVYYCQQYGSSPYTFGQGTKLEIKRADAAPTVSI 48
3-6 3-20/3 EPEDFAVYYCQQYGSSiFTFGPGTKVDIKRADAAPTVSI 49
Claims (64)
1. A mouse comprising, in its germline genome: exactly two unrearranged human V gene segments and five unrearranged human J gene segments operably linked to a mouse light chain constant region at the endogenous kappa light chain loci of the mouse, wherein the exactly two unrearranged human Vκ gene segments are a human Vκ1-39 gene segment and a human Vκ3-20 gene segment; and one or more unrearranged human V gene segments, one or more unrearranged human D gene segments, and one or more unrearranged human J gene segments operably linked to a mouse heavy chain constant region at the endogenous heavy chain loci of the mouse; wherein the unrearranged human heavy chain and kappa light chain gene segments are capable of rearranging and encoding human variable domains of an antibody, and further wherein the mouse does not comprise an endogenous V gene segment that is capable of rearranging to form an immunoglobulin light chain variable region.
2. The mouse of claim 1, wherein the mouse light chain constant region gene is a rat C region gene.
3. The mouse of claim 1, wherein the five unrearranged human immunoglobulin J gene segments of the mouse are a human J 1 gene segment, a human J 2 gene segment, a human J 3 gene segment, a human J4 gene segment, and a human J 5 gene segment.
4. The mouse of claim 1, wherein the mouse comprises a functional light chain locus.
5. The mouse of claim 1, wherein the mouse does not comprise a functional light chain locus.
6. An isolated cell of the mouse of claim 1.
7. The cell of claim 6, wherein the cell is a B cell.
8. A hybridoma made with the B cell of claim 7.
9. The mouse of claim 1, wherein the human Vκ1-39 gene segment is a human germline Vκ1-39 gene segment and the human Vκ3-20 gene segment is a human germline Vκ3-20 gene segment.
10. The mouse of claim 1, wherein the germline genome of the mouse comprises in order: the human V 1-39 gene segment, the human V 3-20 gene segment, the human J 1 gene segment, the human J 2 gene segment, the human J 3 gene segment, the human J 4 gene segment, and the human J 5 gene segment.
11. A in vitro method for making an antibody comprising: expressing in a single cell: (a) a first nucleic acid sequence that encodes a first immunoglobulin heavy chain, the first nucleic acid sequence comprising a first human immunoglobulin heavy chain variable region sequence operably linked to a human immunoglobulin heavy chain constant region sequence, wherein the first human immunoglobulin heavy chain variable region sequence is identified from a B cell of a first mouse, and wherein the first mouse has been immunized with a first antigen of interest including a first epitope, and the first mouse comprises in its germline genome: (i) exactly two unrearranged human immunoglobulin V gene segments and five unrearranged human immunoglobulin J gene segments operably linked to a mouse immunoglobulin light chain constant region sequence at the endogenous kappa light chain loci of the mouse, wherein the two unrearranged human immunoglobulin V gene segments are a human V 1-39 gene segment and a human V 3-20 gene segment; and (ii) one or more unrearranged human immunoglobulin V gene segments, one or more unrearranged human immunoglobulin D gene segments, and one or more unrearranged human immunoglobulin J gene segments operably linked to a mouse immunoglobulin heavy chain constant region sequence at the endogenous heavy chain loci of the mouse; wherein the unrearranged human heavy chain and kappa light chain immunoglobulin gene segments of the first mouse are capable of rearranging and encoding human immunoglobulin variable domains of an antibody, wherein the first mouse does not comprise an endogenous immunoglobulin V gene segment that is capable of rearranging to form an immunoglobulin light chain variable region sequence, and wherein the first human immunoglobulin heavy chain variable region sequence encodes a first human immunoglobulin heavy chain variable domain that recognizes the first epitope; and (b) a second nucleic acid sequence that encodes an immunoglobulin light chain, the second nucleic acid sequence comprising a human immunoglobulin kappa light chain variable region sequence fused with a human immunoglobulin light chain constant region sequence, wherein the human immunoglobulin kappa light chain variable region sequence comprises a human V 1-39 gene segment, a human V 3- 20 gene segment, or a somatically hypermutated version thereof; maintaining the cell in vitro under conditions sufficient to express a fully human antibody; and isolating the antibody.
12. The method of claim 11, wherein the five unrearranged human immunoglobulin J gene segments of the first mouse are a human J 1 gene segment, a human J 2 gene segment, a human J 3 gene segment, a human J 4 gene segment, and a human J 5 gene segment.
13. The method of claim 11, wherein the germline genome of the first mouse comprises in order: the human V 1-39 gene segment, the human V 3-20 gene segment, the human J 1 gene segment, the human J 2 gene segment, the human J 3 gene segment, the human J 4 gene segment, and the human J 5 gene segment.
14. The method of claim 11, wherein the first mouse comprises a functional λ light chain locus.
15. The method of claim 11, wherein the first mouse comprises a nonfunctional λ light chain locus.
16. The method according to claim 11, where the cell comprises a third nucleic acid sequence that encodes a second immunoglobulin heavy chain, the third nucleic acid sequence comprising a second human immunoglobulin heavy chain variable region sequence operably linked to a human immunoglobulin heavy chain constant region sequence, wherein the second human immunoglobulin heavy chain variable region sequence is identified from a B cell of a second mouse, and wherein the second mouse has been immunized with a second antigen of interest including a second epitope and the second mouse comprises in its germline genome: (i) exactly two unrearranged human immunoglobulin V gene segments and five unrearranged human immunoglobulin J gene segments operably linked to a mouse immunoglobulin light chain constant region sequence at the endogenous kappa light chain loci of the mouse, wherein the two unrearranged human immunoglobulin V gene segments are a human V 1-39 gene segment and a human V 3-20 gene segment; and (ii) one or more unrearranged human immunoglobulin V gene segments, one or more unrearranged human immunoglobulin D gene segments, and one or more unrearranged human immunoglobulin J gene segments operably linked to a mouse immunoglobulin heavy chain constant region sequence at the endogenous heavy chain loci of the mouse; wherein the unrearranged human heavy chain and kappa light chain immunoglobulin gene segments of the second mouse are capable of rearranging and encoding human immunoglobulin variable domains of an antibody, and wherein the second human immunoglobulin heavy chain variable region sequence encodes a second human immunoglobulin heavy chain variable domain that recognizes the second epitope, wherein the first epitope and the second epitope are not identical, and wherein the first and the second human immunoglobulin heavy chains pair with the human immunoglobulin light chain encoded by the second nucleic acid sequence.
17. The method of claim 16, wherein the five unrearranged human immunoglobulin J gene segments of the second mouse are a human J 1 gene segment, a human J 2 gene segment, a human J 3 gene segment, a human J 4 gene segment, and a human J 5 gene segment.
18. The method of claim 16, wherein the germline genome of the second mouse comprises in order: the human V 1-39 gene segment, the human V 3-20 gene segment, the human J 1 gene segment, the human J 2 gene segment, the human J 3 gene segment, the human J 4 gene segment, and the human J 5 gene segment.
19. The method of claim 16, wherein the first antigen of interest and the second antigen of interest are the same antigen of interest, and the first and the second epitope are different epitopes on the same antigen.
20. The method of claim 16 wherein the first mouse and the second mouse are the same mouse.
21. The method of claim 16, wherein the human Vκ1-39 gene segment in the germline genome of the first and/or second mouse is a human germline Vκ1-39 gene segment and the human Vκ3-20 gene segment in the germline genome of the first and/or second mouse is a human germline Vκ3-20 gene segment.
22. A method for generating a human heavy and/or kappa light chain variable region sequence comprising: (a) immunizing a genetically modified mouse with an antigen, wherein the mouse generates antibodies when immunized with the antigen, and wherein the mouse has a germline genome that comprises: (i) two unrearranged human Vκ gene segments and five unrearranged human Jκ gene segments operably linked to a light chain constant region sequence, wherein the two unrearranged human Vκ gene segments are a human Vκ1-39 gene segment and a human Vκ3-20 gene segment, and wherein the five unrearranged human Jκ gene segments are a human Jκ1 gene segment, a human Jκ2 gene segment, a human Jκ3 gene segment, a human Jκ4 gene segment, and a human Jκ5 gene segment; and (ii) one or more unrearranged human V gene segments, one or more unrearranged human DH gene segments, and one or more unrearranged human JH gene segments operably linked to a mouse heavy chain constant region sequence; wherein the unrearranged human heavy chain gene segments and unrearranged human kappa light chain gene segments of the mouse are capable of rearranging and encoding human heavy chain variable domains and human kappa light chain variable domains of an antibody, respectively, and wherein the mouse does not comprise an endogenous Vκ gene segment that is capable of rearranging to form a light chain variable region sequence, and (b) determining a human heavy and/or kappa light chain variable region sequence that encodes a human heavy and/or kappa light chain variable domain of an antibody that specifically binds the antigen and that was generated by the genetically modified mouse.
23. A method for generating a human heavy and/or kappa light chain variable domain sequence comprising: (a) immunizing a genetically modified mouse with an antigen, wherein the mouse generates antibodies when immunized with the antigen, and wherein the mouse has a germline genome that comprises: (i) two unrearranged human Vκ gene segments and five unrearranged human Jκ gene segments operably linked to a light chain constant region sequence, wherein the two unrearranged human Vκ gene segments are a human Vκ1-39 gene segment and a human Vκ3-20 gene segment, and wherein the five unrearranged human Jκ gene segments are a human Jκ1 gene segment, a human Jκ2 gene segment, a human Jκ3 gene segment, a human Jκ4 gene segment, and a human Jκ5 gene segment; and (ii) one or more unrearranged human V gene segments, one or more unrearranged human D gene segments, and one or more unrearranged human J gene segments operably linked to a mouse heavy chain constant region sequence; wherein the unrearranged human heavy chain gene segments and unrearranged human kappa light chain gene segments of the mouse are capable of rearranging and encoding human heavy chain variable domains and human kappa light chain variable domains of an antibody, respectively, and wherein the mouse does not comprise an endogenous Vκ gene segment that is capable of rearranging to form a light chain variable region sequence, and (b) determining a human heavy and/or kappa light chain variable domain sequence of an antibody that specifically binds the antigen and that was generated by the genetically modified mouse.
24. The method of claim 23, wherein determining a human heavy and/or kappa light chain variable domain sequence comprises determining a nucleotide sequence that encodes the human heavy and/or kappa light chain variable domain sequence.
25. The method of claim 22 or 23, wherein the two unrearranged human V gene segments and five unrearranged human J gene segments in the germline genome of the mouse are operably linked to a mouse light chain constant region sequence.
26. The method of claim 25, wherein the mouse light chain constant region sequence is a mouse C region sequence.
27. The method of claim 25, wherein the two unrearranged human V gene segments and five unrearranged human J gene segments in the germline genome of the mouse are present at an endogenous immunoglobulin light chain locus.
28. The method of claim 27, wherein the germline genome of the mouse comprises in order: the human V 1-39 gene segment, the human V 3-20 gene segment, the human J 1 gene segment, the human J 2 gene segment, the human J 3 gene segment, the human J 4 gene segment, and the human J 5 gene segment.
29. The method of claim 22 or 23, wherein the one or more unrearranged human V gene segments, one or more unrearranged human D gene segments, and one or more unrearranged human J gene segments in the germline genome of the mouse are present at the endogenous immunoglobulin heavy chain locus.
30. The method of claim 29, wherein the mouse does not comprise an endogenous mouse immunoglobulin V gene segment that is capable of rearranging to form an immunoglobulin heavy chain variable region.
31. The method of claim 22 or 23, wherein the mouse comprises a nonfunctional immunoglobulin λ light chain locus.
32. A mouse embryonic stem (ES) cell that has been genetically modified so that it comprises in its genome: exactly two unrearranged human immunoglobulin V gene segments and five unrearranged human immunoglobulin J gene segments operably linked to a mouse immunoglobulin light chain constant region sequence, wherein the two unrearranged human immunoglobulin V gene segments are a human V 1-39 gene segment and a human V 3-20 gene segment, and wherein the five unrearranged human immunoglobulin J gene segments are a human J 1 gene segment, a human J 2 gene segment, a human J 3 gene segment, a human J 4 gene segment, and a human J 5 gene segment.
33. The genetically modified mouse ES cell of claim 32, further comprising in its genome: one or more unrearranged human immunoglobulin V gene segments, one or more unrearranged human immunoglobulin D gene segments, and one or more unrearranged human immunoglobulin J gene segments operably linked to a mouse immunoglobulin heavy chain constant region sequence at the endogenous heavy chain loci.
34. The genetically modified ES cell of claim 33, wherein the genome of the ES cell does not comprise an endogenous mouse immunoglobulin V gene segment that is capable of rearranging to form an immunoglobulin heavy chain variable region.
35. The genetically modified ES cell of any one of claims 32 to 34, wherein the two unrearranged human immunoglobulin V gene segments and five unrearranged human immunoglobulin J gene segments are present at the endogenous immunoglobulin light chain locus.
36. The genetically modified ES cell of claim 32 or claim 33, wherein the genome of the genetically modified mouse ES cell does not comprise a functional λ light chain locus.
37. The genetically modified mouse ES cell of claim 32 or claim 33, wherein the mouse light chain constant region is a mouse kappa constant region.
38. The genetically modified mouse ES cell of claim 37, wherein the mouse C constant region is an endogenous mouse C constant region.
39. The genetically modified mouse ES cell of claim 32 or claim 33, wherein the human Vκ1-39 gene segment in genome of the genetically modified mouse ES cell is a human germline Vκ1-39 gene segment and the human Vκ3-20 gene segment in the genome of the genetically modified mouse ES cell is a human germline Vκ3-20 gene segment.
40. The genetically modified mouse ES cell of claim 32 or claim 33, wherein the genome of the genetically modified mouse ES cell comprises in order: the human V 1-39 gene segment, the human V 3-20 gene segment, the human J 1 gene segment, the human J 2 gene segment, the human J 3 gene segment, the human J 4 gene segment, and the human J5 gene segment.
41. The genetically modified mouse ES cell of any one of claims 32 to 40, wherein the genome of the genetically modified mouse ES cell comprises a DLC-5J locus, wherein the DLC-5J locus comprises a hV /hJ /mC junction sequence selected from SEQ ID NOs: 38-49.
42. A mouse embryo derived from the genetically modified ES cell of claim 32 or claim 33.
43. A method of making a mouse comprising gestating the mouse embryo of claim 42 in a surrogate mother, and allowing the surrogate mother to give birth to progeny derived in whole or in part from the genetically modified ES cell.
44. A method of making a genetically modified mouse ES cell, the method comprising genetically modifying an ES cell so that it comprises in its genome exactly two unrearranged human immunoglobulin V gene segments and five unrearranged human immunoglobulin J gene segments operably linked to a mouse immunoglobulin light chain constant region sequence, wherein the two unrearranged human immunoglobulin V gene segments are a human V 1-39 gene segment and a human V 3-20 gene segment, and wherein the five unrearranged human immunoglobulin J gene segments are a human J 1 gene segment, a human J 2 gene segment, a human J 3 gene segment, a human J 4 gene segment, and a human J 5 gene segment.
45. The method of claim 44, wherein the genetically modified mouse ES cell further comprises in its genome one or more unrearranged human immunoglobulin V gene segments, one or more unrearranged human immunoglobulin D gene segments, and one or more unrearranged human immunoglobulin J gene segments operably linked to a mouse immunoglobulin heavy chain constant region sequence at the endogenous heavy chain loci.
46. The method of claim 44 or claim 45, wherein the mouse light chain constant region is a mouse C constant region.
47. The method of claim 46, wherein the mouse light chain constant region is an endogenous mouse C constant region.
48. The method of claim 45, wherein the genome of the genetically modified ES cell does not comprise an endogenous mouse immunoglobulin V gene segment that is capable of rearranging to form an immunoglobulin heavy chain variable region.
49. The method of any one of claims 44 to 48, wherein the two unrearranged human immunoglobulin V gene segments and five unrearranged human immunoglobulin J gene segments are present at the endogenous immunoglobulin light chain locus.
50. The method of claim 44 or claim 45, wherein the genome of the genetically modified mouse ES cell does not comprise a functional λ light chain locus.
51. The method of claim 44 or claim 45, wherein the human Vκ1-39 gene segment in the genome of the genetically modified mouse ES cell is a human germline Vκ1-39 gene segment and the human Vκ3-20 gene segment in the genome of the genetically modified mouse ES cell is a human germline Vκ3-20 gene segment.
52. The method of claim 44 or claim 45, wherein the genome of the genetically modified mouse ES cell comprises in order: the human V 1-39 gene segment, the human V 3-20 gene segment, the human J 1 gene segment, the human J 2 gene segment, the human J 3 gene segment, the human J 4 gene segment, and the human J 5 gene segment.
53. The method of any one of claims 44 to 52, wherein the genetically modified mouse ES cell comprises a DLC-5J locus, wherein the DLC-5J locus comprises a hV /hJ /mC junction sequence selected from SEQ ID NOs: 38-49.
54. A method of making a genetically modified mouse comprising genetically modifying the germline genome of the mouse so that it includes exactly two unrearranged human immunoglobulin V gene segments and five unrearranged human immunoglobulin J gene segments operably linked to a mouse immunoglobulin light chain constant region sequence, wherein the two unrearranged human immunoglobulin V gene segments are a human V 1- 39 gene segment and a human V 3-20 gene segment, and wherein the five unrearranged human immunoglobulin J gene segments are a human J 1 gene segment, a human J 2 gene segment, a human J 3 gene segment, a human J 4 gene segment, and a human J 5 gene segment.
55. The method of claim 54, wherein the genetically modified mouse further comprises in its genome one or more unrearranged human immunoglobulin V gene segments, one or more unrearranged human immunoglobulin D gene segments, and one or more unrearranged human immunoglobulin J gene segments operably linked to a mouse immunoglobulin heavy chain constant region sequence at the endogenous heavy chain loci.
56. The method of claim 54 or claim 55, wherein the mouse light chain constant region is a mouse C constant region.
57. The method of claim 56, wherein the mouse light chain constant region is an endogenous mouse C constant region.
58. The method of claim 55, wherein the genome of the genetically modified mouse does not comprise an endogenous mouse immunoglobulin V gene segment that is capable of rearranging to form an immunoglobulin heavy chain variable region.
59. The method of any one of claims 54 to 58, wherein the two unrearranged human immunoglobulin V gene segments and five unrearranged human immunoglobulin J gene segments are present at the endogenous immunoglobulin light chain locus.
60. The method of claim 54 or claim 55, wherein the genome of the genetically modified mouse comprises a nonfunctional immunoglobulin λ light chain locus.
61. The method of claim 54 or claim 55, wherein the genome of the genetically modified mouse does not comprise a functional λ light chain locus.
62. The method of claim 54 or claim 55, wherein the human Vκ1-39 gene segment in the genome of the genetically modified mouse is a human germline Vκ1-39 gene segment and the human Vκ3-20 gene segment in the genome of the genetically modified mouse is a human germline Vκ3-20 gene segment.
63. The method of claim 54 or claim 55, wherein the genome of the genetically modified mouse comprises in order: the human V 1-39 gene segment, the human V 3-20 gene segment, the human J 1 gene segment, the human J 2 gene segment, the human J 3 gene segment, the human J 4 gene segment, and the human J 5 gene segment.
64. The method of any one of claims 54 to 63, wherein the genetically modified mouse comprises a DLC-5J locus, wherein the DLC-5J locus comprises a hV /hJ /mC junction sequence selected from SEQ ID NOs: 38-49.
Applications Claiming Priority (3)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| US13/798,455 US9796788B2 (en) | 2010-02-08 | 2013-03-13 | Mice expressing a limited immunoglobulin light chain repertoire |
| US13/798,455 | 2013-03-13 | ||
| PCT/US2014/026040 WO2014160202A1 (en) | 2013-03-13 | 2014-03-13 | Mice expressing a limited immunoglobulin light chain repertoire |
Publications (2)
| Publication Number | Publication Date |
|---|---|
| NZ711776A NZ711776A (en) | 2021-09-24 |
| NZ711776B2 true NZ711776B2 (en) | 2022-01-06 |
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